Patent Application
20080032921
This application includes a “Sequence Listing,” which is provided as an electronic document on a compact disc (CD-R). This compact disc contains the file “Sequence Listing.txt” (129,024 bytes, created on May 18, 2007), which is herein incorporated by reference in its entirety.
The present invention relates to influenza virus vaccine compositions and methods of treating or preventing influenza infection and disease in mammals. Influenza is caused by an RNA virus of the myxovirus group. Influenza viruses can be classified into three types (A, B and C), based on antigenic differences in the nucleoprotein and the matrix protein. Type A, which includes several subtypes, causes widespread epidemics and global pandemics. Type B causes regional epidemics. Influenza C is less severe and has been isolated from humans and pigs. Type C causes sporadic cases and minor, local outbreaks. Influenza A viruses can be further classified based on the viral surface proteins hemagglutinin (HA or H) and neuraminidase (NA or N). There are sixteen known H subtypes and nine known N subtypes of Type A viruses; while there is only one known H subtype and one N subtype of Type B viruses. Typical nomenclature identifies an influenza virus by both proteins, e.g., H3N2.
Type A and B influenza viruses each contain 8 RNA segments, while type C only has 7 RNA segments. Influenza A is most important and is very pathogenic for man, as well as for animals, for example pigs and horses. Type B influenza causes disease in humans. These virus types are distinguished in part on the basis of differences in two structural proteins, the nucleoprotein, found in the center of the virus, and the matrix protein, which forms the viral shell. The virus is transmitted through the air, mainly in droplets expelled during coughing and sneezing. The influenza viruses cause an infection of the respiratory tract, which is usually accompanied with coughing, high fever and myalgia.
Although an influenza infection does not often lead to the death of the infected individual, the morbidity can be severe. As a consequence thereof influenza epidemics may lead to substantial economic loss. Furthermore, influenza infection can be more dangerous for certain groups of individuals, such as those having suffered from a heart attack, CARA patients or the elderly. A vaccine against influenza is therefore highly desirable.
Influenza Epidemiology and Virology
Pandemics of influenza A viruses continue to occur at sporadic intervals in human populations. Three have occurred in the twentieth century alone in 1918, 1957 and 19686-8. These worldwide pandemics are noted for their high mortality with rates approaching 30-50%9. For example, it is estimated that 20-40 million people died in the 1918 pandemic and at least 1.5 million people in the 1957 and 1968 outbreaks combined10. Whether a pandemic occurs from an act of nature or from the deliberate release of a novel influenza strain with pandemic potential, the extent of world travel will ensure the rapid global spread of the pandemic agent. Such an event could result in world-wide deaths totaling in the millions and severely impact health care systems such that economies and governments of smaller countries could collapse9,11.
The capacity of the influenza virus to cause disease in a recurring manner is due to a complex set of factors that include: 1) the presence of an established reservoir of influenza A viruses of different subtypes in shorebirds and waterfowl; 2) the ability of avian influenza viruses to recombine with influenza viruses of other animals, most notably swine12, a process termed ‘antigenic shift’; 3) accumulation of mutations in viral gene products caused by a lack of proofreading activity of the viral RNA polymerase, a process termed ‘antigenic drift’. These reassortment and mutation events combine to cause the well-characterized antigenic variability in the two surface glycoproteins of the virus, hemagglutinin (HA) and neuraminidase (NA)13-15 which provides the virus a mechanism for escaping immune responses, particularly neutralizing antibodies, induced as the result of previous infections or vaccinations. Antigenic shift, which occurs only among influenza A viruses, results in major antigenic change introducing viruses with a new gene segment(s). Antigenic shift can occur when an animal influenza A virus is transmitted directly to humans, such as the transmission of the H1N1 from swine-to-human16 or the transmission of the H5N1, H7N7 or H9N2 variants from avian to human17,18. Alternatively, a virus may acquire a new gene segment(s) as a result of genetic reassortment between animal and human influenza A viruses, the cause of the 1957 H2N2 and 1968 H3N2 pandemics19.
Since 1997, several novel avian subtypes have crossed the so-called species barrier from domestic poultry to humans and have caused a spectrum of mild to severe and even fatal human disease. In 1997, 18 cases of human infection with highly pathogenic avian H5N1 influenza viruses, including 6 deaths were documented in Hong Kong following outbreaks of disease in domestic poultry. Avian H5N1 viruses reemerged in Hong Kong and from Dec. 30, 2003 to Mar. 17, 2004, there were 12 human cases of confirmed H5N1 influenza in Thailand and 23 in Vietnam, including 23 deaths. As of May 2006, approximately 115 deaths have been attributed to H5N1 infection. The H5N1 strain does not jump easily from birds to humans or between humans. However since the human virus, H3N2, can coexist with avian influenza viruses and is widespread in pigs from southeast China, reassortment has the potential to occur with a highly pathogenic human-to-human transmissible H5N1 being the result. Although these wholly avian viruses were associated with only limited human-to-human transmission, their repeated emergence in humans highlights the potential for the generation of an avian-human reassortant virus with the potential for spread in the human population. Thus, the development of effective vaccines against these avian subtypes is of the highest public health priority.
Vaccine production must rely on surveillance programs to predict the influenza subtypes likely to have global impact on human health. The time required to produce subtype-matched vaccines, composed of inactivated or ‘split’ virions, typically requires a minimum of 6-8 months. In the face of a serious influenza virus pandemic caused by a viral subtype, this lag time could allow for national or international spread with excessive morbidity and mortality.
Virus Structures
An influenza virus is roughly spherical, but it can also be elongated or irregularly shaped. Inside the virus, eight segments of single-stranded RNA contain the genetic instructions for making the virus. The most striking feature of the virus is a layer of spikes projecting outward over its surface. There are two different types of spikes: one is composed of the molecule hemagglutinin (HA), the other of neuraminidase (NA). The HA molecule allows the virus to “stick” to a cell, initiating infection. The NA molecule allows newly formed viruses to exit their host cell without sticking to the cell surface or to each other. The viral capsid is comprised of viral ribonucleic acid and several so called “internal” proteins (polymerases (PB1, PB2, and PA, matrix protein (M1) and nucleoprotein (NP)). Because antibodies against HA and NA have traditionally proved the most effective in fighting infection, much research has focused on the structure, function, and genetic variation of those molecules. Researchers are also interested in two non-structural proteins M2 and NS1; both molecules play important roles in viral infection.
Type A subtypes are described by a nomenclature system that includes the geographic site of discovery, a lab identification number, the year of discovery, and in parentheses the type of HA and NA it possesses, for example, A/Hong Kong/156/97 (H5N1). If the virus infects non-humans, the host species is included before the geographical site, as in A/Chicken/Hong Kong/G9/97 (H9N2).
Virions contain 7 segments (influenza C virus) to 8 segments (influenza A and B virus) of linear negative-sense single stranded RNA. Most of the segments of the virus genome code for a single protein. For many influenza viruses, the whole genome is now known. Genetic reassortment of the virus results from intermixing of the parental gene segments in the progeny of the viruses when a cell is co-infected by two different viruses of a given type. This phenomenon is facilitated by the segmental nature of the genome of influenza virus. Genetic reassortment is manifested as sudden changes in the viral surface antigens.
Antigenic changes in HA and NA allow the influenza virus to have tremendous variability. Antigenic drift is the term used to indicate minor antigenic variations in HA and NA of the influenza virus from the original parent virus, while major changes in HA and NA which make the new virions significantly different, are called Antigenic shift. The difference between the two phenomena is a matter of degree.
Antigenic drift (minor changes) occurs due to accumulation of point mutations in the gene which results in changes in the amino acids in the proteins. Changes which are extreme, and drastic (too drastic to be explained by mutation alone) result in antigenic shift of the virus. The segmented genomes of the influenza viruses reassort readily in double infected cells. Genetic reassortment between human and non-human influenza virus has been suggested as a mechanism for antigenic shift. Influenza is a zoonotic disease, and an important pathogen in a number of animal species, including swine, horses, and birds, both wild and domestic. Influenza viruses are transferred to humans from other species.
Because of antigenic shift and antigenic drift, immunity to an influenza virus carrying a particular HA and/or NA protein does not necessarily confer protective immunity against influenza virus strains carrying variant, or different HA and/or NA proteins. Because antibodies against HA and NA have traditionally proved the most effective in fighting influenza virus infection, much research has focused on the structure, function and genetic variation of those molecules.
Role of Cellular Immune Responses in Protection Against Influenza
Cellular immune responses are known to contribute to the control of viral replication in vivo and to mediate viral clearance. In murine models, influenza-specific CD8+ cytotoxic T-lymphocytes (CTL) limit virus replication and protect against lethal virus challenge20-27. Recovery from infection correlated with virus-specific CD8+ CTL activity22 and lack of CD8+ CTL activity was associated with delayed viral clearance and increased mortality28. Studies completed by Ulmer and Okuda using a DNA vaccine encoding the viral nucleoprotein and M gene proteins, respectively are particularly relevant. These vaccines induced influenza-specific CD8+ CTL that provided cross-strain protection27,29,30. The contribution of CTL and Helper T-lymphocytes (HTL) was definitively demonstrated by adoptive transfer of CD8+ and CD4+ T-lymphocytes31. Similarly, Epstein and colleagues demonstrated that either CD8+ or CD4+ T-lymphocytes promoted survival in mice immunized with an experimental DNA vaccine encoding internal viral proteins32. Finally, virus specific HTL augment the generation of CTL and size of the CTL memory pool, an effect known to be associated with long term protection33. Cellular immune responses clearly contribute to the control and clearance of infection and reduce pathogenesis.
The exposure to an influenza virus of one subtype often induces immune responses that protect against infection or disease with another subtype, a phenomena referred to as Heterosubtypic Immunity (HSI)34-37. The mechanisms of heterosubtypic immunity appears to involve functional activity of both CD8+ and CD4+ T-lymphocytes23,26,38-41, although more recently antibody responses have also been implicated42. HSI is not only observed using the murine models; influenza virus-specific CTL appear to provide partial protection against multiple influenza A virus strains in humans. Early human studies demonstrated that cellular immune responses play a role in controlling influenza infection43,44. McMichael and colleagues inoculated 63 volunteers intranasally with live unattenuated influenza A/Munich/l/79 virus and evaluated the protective effects of serum antibody and cytotoxic T-cell immunity against influenza.43 It was found that all subjects with demonstrable T-cell responses cleared virus effectively. Sonoguchi and colleagues found that students previously infected with H3N2 virus were partially protected against subsequent infection with H1N1 subtype virus suggesting cross-subtype protection in humans during sequential epidemics. Thus, the use of vaccines to induce cellular responses against pandemic influenza virus is logical and the development of suitable vaccine technologies is warranted.
Immune system-mediated selection pressure on influenza virus can lead to CTL viral escape mutants45-47. While this phenomena clearly documents the importance of virus-specific CTL it also reveals a potential limitation for vaccines designed to induce CTL responses. However, the use of carefully selected epitopes in the design of a vaccine provides a means to address this problem. Selection of epitopes that are highly conserved amongst multiple viral strains is the first step and the selection of those epitopes predicted to be capable of inducing CTL responses to the majority of related epitopes is the second step.
Role of Humoral Immune Responses in Protection Against Influenza
Influenza vaccines are formulated to include human influenza strains predicted to pose the greatest risk for infectious spread. This vaccine development process requires approximately 6-8 months using conventional strains. Neutralizing antibodies induced primarily to the surface hemagglutinin protein by the conventional vaccines are highly protective. However, due to antigenic drift of the virus, the vaccines must be reformulated on a yearly basis. The danger persists that a “new” strain will emerge by antigenic shift for which the human population has little or no pre-existing immunity. Also, since vaccine production relies on embryonated chicken eggs or potentially cells in tissue culture, there are no assurances that sufficient new virus can be produced even within the 6-8 month time frame especially if the new influenza strain is lethal to birds. Pandemic influenza vaccine development would benefit by inclusion of conserved B cell epitopes capable of inducing protective immune responses. To this end, it has been reported that the external domain of the transmembrane viral M2 protein is highly conserved and that antibodies directed to this epitope are protective in mice48-54. The M2 protein is an integral membrane protein of influenza A virus that is expressed at the plasma membrane in virus-infected cells. Due to the low abundance of the protein in the virus, the mechanism of protection of the antibody response directed against this epitope is not mediated via viral neutralization but rather by antibody-dependent, cell-mediated cytotoxicity51.
Conserved CTL, HTL and B-cell epitopes can be used as the basis for a vaccine designed to augment and improve prototype pandemic vaccine candidates that may be poorly immunogenic or a sub-optimal match against a pandemic strain that emerges. The advantages to using defined epitopes in vaccines are many but one advantage is that many epitopes can be incorporated into a vaccine to induce a broadly specific immune response targeting numerous viral gene products. Data from natural infection studies wherein human memory CTL specific to influenza A virus were restricted by multiple HLA Class I alleles have shown that responses within a given individual were broadly directed to epitopes within the NP, NA, HA, M1, NS1 and M2 viral proteins.
Design and Testing of Vaccines to Induce Cellular and Humoral Immune Responses:
The use of recombinant DNA technology to produce influenza vaccines offers several advantages: a recombinant DNA influenza vaccine can be produced under safer and more stringently controlled conditions; propagation with infectious influenza in eggs is not required; recombinant HA protein can be more highly purified, virtually eliminating side effects due to contaminating proteins; purification procedures for recombinant HA do not have to include virus inactivation or organic extraction of viral membrane components, therefore avoiding denaturation of antigens and additional safety concerns due to residual chemicals in the vaccine. Production of HA via recombinant DNA technology provides an opportunity to avoid the genetic heterogeneity which occurs during adaptation and passage through eggs, which should make it possible to better match vaccine stains with influenza epidemic strains, resulting in improved efficacy; and a recombinant approach may also allow for strain selection later in the year, thereby allowing time for selections based on more reliable epidemiological data.
A major obstacle to the development of vaccines that induce immune responses is the selection of a suitable delivery format. DNA plasmid vaccines and viral vectors, used either alone or together, and recombinant protein or peptides are logical vaccine delivery formats; however, each format has advantages and disadvantages. For example, DNA vaccines are readily produced and safe to administer but potency has been lacking, especially in clinical trials, requiring the administration of large (milligram) doses59-65. Studies completed in small animals have indicated increased vaccine potency66-69. Polymer formulation technology based on polyvinylpyrrolidone (PVP) can also be utilized. PVP is a nontoxic formulation excipient used to enhance DNA plasmid uptake by muscle cells70-73. Such vaccine design parameters can correct for at least some of the limitations of naked-DNA vaccine technology.
The use of viral vectors to deliver vaccines has raised concerns, usually related to safety and pre-existing immunity to the vector. However, AlphaVax replicons are reported to be safe, non-transmissible and there is a general lack of pre-existing immunity to the vector. Another delivery vehicle that is being evaluated is peptides in adjuvant. Generally, peptides in adjuvant have shown to be immunogenic and efficacious in humans. However, there are concerns regarding vaccine formulation wherein high numbers of peptides will need to be delivered.
Several adjuvants have been developed for the administration of influenza virus vaccines, including alum based compounds, emulsions (e.g. MF59), (lipophilic immune stimulating complexes ISCOMS) containing Quil A adjuvant) and liposomes. A development of the liposomal technique has been the use of immunopotentiating reconstituted influenza virosomes (IRIVs) as antigen delivery systems. See Mischler, R. and Metcalfe, I. C., Vaccine 20: B17-B23 (2002). The IRIV vaccine delivery system is comprised of spherical unilamellar vesicles comprising naturally occurring phospholipids (PL) and phosphatidylcholine (PC) and envelope phospholipids originating from influenza virus used to provide influenza virus NA and HA glycoproteins. See id. The fusion mechanism of IRIVs enables stimulation of the MHC Class I or Class II pathway, depending upon how antigens are presented to the APCs. Virosomes are able to induce either a B- or T-cell response. See id.
The use of smaller polypeptides comprising antigenic epitopes in vaccines has several advantages over current vaccines, particularly when compared to the use of whole antigens in vaccine compositions. There is evidence that the immune response to whole antigens is directed largely toward variable regions of the antigen, allowing for immune escape due to mutations. The epitopes for inclusion in an epitope-based vaccine may be selected from conserved regions of influenza antigens, which thereby reduces the likelihood of escape mutants. Furthermore, immunosuppressive epitopes that may be present in whole antigens can be avoided with the use of epitope-based vaccines.
An additional advantage of an epitope-based vaccine approach is the ability to combine selected epitopes (e.g., multiple HTL epitope epitopes), and further, to modify the composition of the epitopes, achieving, for example, enhanced immunogenicity. Accordingly, the immune response can be modulated, as appropriate, for the target disease. Similar engineering of the response is not possible with traditional approaches.
Several groups have established the mouse model as a tool for evaluating the efficacy of influenza vaccines26-31,74,75. The testing of vaccines comprised of epitopes restricted by HLA is a unique challenge, requiring the appropriate restriction elements. Specifically cell-surface expressed HLA Class II molecules for HTL epitopes on antigen presenting cells are required. With regard to evaluating Class II-restricted responses, HLA-DR4 mice are available commercially. Most HTL epitopes restricted to HLA Class II can bind murine H-2 IAb molecules and initiate a response80.
Virus-specific, human leukocyte antigen (HLA) class I-restricted cytotoxic T lymphocytes (CTL) are known to play a major role in the prevention and clearance of virus infections in vivo (Oldstone, et al., Nature 321:239, 1989; Jamieson, et al., J. Virol. 61:3930, 1987; Yap, et al., Nature 273:238, 1978; Lukacher, et al., J. Exp. Med. 160:814, 1994; McMichael, et al., N. Engl. J. Med. 309:13, 1983; Sethi, et al., J. Gen. Virol. 64:443, 1983; Watari, et al., J. Exp. Med. 165:459, 1987; Yasukawa, et al., J. Immunol. 143:2051, 1989; Tigges, et al., J. Virol. 66:1622, 1993; Reddenhase, et al., J. Virol. 55:263, 1985; Quinnan, et al., N. Engl. J. Med. 307:6, 1982). HLA class I molecules are expressed on the surface of almost all nucleated cells. Following intracellular processing of antigens, epitopes from the antigens are presented as a complex with the HLA class I molecules on the surface of such cells. CTL recognize the peptide-HLA class I complex, which then results in the destruction of the cell bearing the HLA-peptide complex directly by the CTL and/or via the activation of non-destructive mechanisms e.g., the production of interferon, that inhibit viral replication.
Virus-specific T helper lymphocytes are also known to be critical for maintaining effective immunity in chronic viral infections. Historically, HTL responses were viewed as primarily supporting the expansion of specific CTL and B cell populations; however, more recent data indicate that HTL may directly contribute to the control of virus replication. For example, a decline in CD4+ T cells and a corresponding loss in HTL function characterize infection with HIV (Lane, et al., N. Engl. J. Med. 313:79, 1985). Furthermore, studies in HIV infected patients have also shown that there is an inverse relationship between virus-specific HTL responses and viral load, suggesting that HTL plays a role in controlling viremia (see, e.g., Rosenberg, et al., Science 278:1447, 1997).
The epitope approach, as we describe herein, allows the incorporation of various antibody, CTL and HTL epitopes, from various proteins, in a single vaccine composition. Such a composition may simultaneously target multiple dominant and subdominant epitopes and thereby be used to achieve effective immunization in a diverse population.
The technology relevant to multi-epitope (“minigene”) vaccines is developing. Several independent studies have established that induction of simultaneous immune responses against multiple epitopes can be achieved. For example, responses against a large number of T cell specificities can be induced and detected. In natural situations, Doolan, et al. (Immunity, Vol. 7(1):97-112 (1997)) simultaneously detected recall T cell responses, against as many as 17 different P. falciparum epitopes using PBMC from a single donor. Similarly, Bertoni and colleagues (J. Clin. Invest., 100(3):503-13 (1997)) detected simultaneous CTL responses against 12 different HBV-derived epitopes in a single donor. In terms of immunization with multi-epitope nucleic acid vaccines, several examples have been reported where multiple T cell responses were induced. For example, minigene vaccines composed of approximately ten MHC Class I epitopes in which all epitopes were immunogenic and/or antigenic have been reported. Specifically, minigene vaccines composed of 9 EBV (Thomson, et al., Proc. Natl. Acad. Sci. USA, 92(13):5845-49 (1995)), 7 HIV (Woodberry, et al., J. Virol., 73(7):5320-25 (1999)), 10 murine (Thomson, et al., J. Immunol., 160(4):1717-23 (1998)) and 10 tumor-derived (Mateo, et al., J. Immunol., 163(7):4058-63 (1999)) epitopes have been shown to be active. It has also been shown that a multi-epitope DNA plasmid encoding nine different HLA-A2.1- and A11-restricted epitopes derived from HBV and HIV induced CTL against all epitopes (Ishioka, et al., J. Immunol., 162(7):3915-25 (1999)).
Recently, several multi-epitope DNA plasmid vaccines specific for HIV have entered clinical trials (Nanke, et al., Nature Med., 6:951-55 (2000); Wilson, C. C., et al., J. Immunol. 171(10):5611-23 (2003).
Thus, vaccines containing multiple MHC Class I and Class II (i.e., HTL) epitopes can be designed, and presentation and recognition can be obtained for all epitopes. However, the immunogenicity of such multi-epitope constructs appears to be strongly influenced by a number of variables, a number of which have heretofore been unknown. For example, the immunogenicity (or antigenicity) of the same epitope expressed in the context of different vaccine constructs can vary over several orders of magnitude. Thus, there exists a need to identify strategies to optimize such multi-epitope containing vaccine constructs. Such optimization is important in terms of induction of potent immune responses and ultimately, for clinical efficacy. Accordingly, the present invention provides strategies to optimize antigenicity and immunogenicity of multi-epitope vaccines encompassing a certain number of epitopes. The present invention also provides optimized multi-epitope containing vaccines, particularly minigene vaccines, generated in accordance with these strategies.
The present invention is directed to enhancing the immune response of a vertebrate in need of protection against influenza virus infection by administering in vivo, into a tissue of the vertebrate, at least one polynucleotide, wherein the polynucleotide comprises a nucleic acid sequence of a coding region operably encoding an influenza virus polypeptide, or fragment, variant, or derivative thereof and a pan-DR binding epitope (e.g. PADRE®). The polynucleotide of the present invention can further comprise one or more nucleic acids encoding a helper T lymphocyte (HTL) epitope.
In certain embodiments, the invention provides a polynucleotide comprising (a) a nucleic acid encoding zero to ten HTL epitopes; (b) a nucleic acid encoding a pan-DR binding epitope; (c) a nucleic acid encoding an influenza virus hemagglutinin (HA) sequence, or fragment thereof; and (d) optionally, a nucleic acid encoding an influenza matrix protein 2 external (M2e) sequence, or fragment thereof. In other embodiments, the invention provides a polynucleotide comprising (a) a nucleic acid encoding zero to ten HTL epitopes; (b) a nucleic acid encoding a pan-DR binding epitope; (c) a nucleic acid encoding an influenza virus matrix protein 2 external (M2e) sequence, or fragment thereof; and (d) optionally, a nucleic acid encoding an influenza virus hemagglutinin (HA) sequence, or fragment thereof. In further embodiments, the polynucleotide of the invention encodes a polypeptide comprising the pan-DR-binding epitope AKFVAAWTLKAAA (SEQ ID NO:1). In certain embodiments, the pan-DR binding epitope may be located on either the 5′ or 3′ end of the polynucleotide encoding an influenza virus hemagglutinin sequence, or fragment thereof, or positioned within an influenza virus hemagglutinin sequence, or fragment thereof as a straight insertion between influenza amino acids or as a replacement of influenza amino acids. In further embodiments, the nucleic acids of (a), (b), (c), and optionally (d), can be arranged in any order relative to one another.
In certain embodiments, the polynucleotide comprises a nucleic acid encoding zero to seven HTL epitopes. In other embodiments, the polynucleotide comprises a nucleic acid encoding zero to five HTL epitopes. In further embodiments, the polynucleotide comprises a nucleic acid encoding zero to four HTL epitopes. In further embodiments, the polynucleotide comprises a nucleic acid encoding zero to three HTL epitopes. In further embodiments, the polynucleotide comprises a nucleic acid encoding zero to two HTL epitopes. In further embodiments, the polynucleotide comprises a nucleic acid encoding zero to one HTL epitopes.
The polynucleotide of the invention can comprise a nucleic acid of a coding region operably encoding any influenza polypeptide or fragment, variant, or, derivative thereof, including, but not limited to, HA, NA, NP, PA, PB1, PB2, NS1, NS2, M1 or M2 proteins or fragments (e.g., M2e), variants or derivatives thereof. A polynucleotide of the invention can also encode a derivative fusion protein, wherein two or more nucleic acid fragments, at least one of which encodes an influenza polypeptide or fragment, variant, or derivative thereof, are joined in frame to encode a single polypeptide, e.g., HA fused to M2e. Additionally, a polynucleotide of the invention can further comprise a heterologous nucleic acid or nucleic acid fragment. Such heterologous nucleic acid or nucleic acid fragment may encode a heterologous polypeptide fused in frame with the polynucleotide encoding the influenza virus polypeptide, e.g., a hepatitis B core protein or a secretory signal peptide. Preferably, the polynucleotide encodes an influenza polypeptide or fragment, variant, or derivative thereof comprising at least one immunogenic epitope of influenza virus, wherein the epitope elicits a B-cell (antibody) response, a T-cell response, or both.
In certain embodiments, the invention provides a polypeptide comprising (a) a polypeptide encoding zero to ten HTL epitopes; (b) a pan-DR binding epitope; (c) an influenza virus hemagglutinin (HA) sequence, or fragment thereof; and (d) optionally, an influenza matrix protein 2 external (M2e) sequence, or fragment thereof. In other embodiments, the invention provides a polypeptide comprising (a) a polypeptide having from zero to ten HTL epitopes; (b) a pan-DR binding epitope; (c) an influenza virus matrix protein 2 external (M2e) sequence, or fragment thereof; and (d) optionally, an influenza virus hemagglutinin (HA) sequence, or fragment thereof. In polypeptide embodiments, the pan-DR-binding epitope comprises the amino acid sequence a1KXVAAWTLKAAa2 (SEQ ID NO:2), where “X” is selected from the group consisting of cyclohexylalanine, phenylalanine, and tyrosine; and “a1” is either D-alanine or L-alanine; and “a2” is either D-alanine or L-alanine. In alternative embodiments, the pan-DR binding epitope may be located on the N- or C-terminus of the polypeptide of the present invention, or positioned within an influenza sequence as a straight insertion between influenza amino acids or as a replacement of influenza amino acids. In further embodiments, polypeptides of (a), (b), (c), and optionally (d), can be arranged in any order relative to one another.
Similarly, the isolated influenza polypeptide, fragment, variant, or derivative thereof to be delivered (either a recombinant protein, a purified subunit, or viral vector expressing an isolated influenza polypeptide, or in the form of an inactivated influenza vaccine) can be any isolated influenza virus polypeptide or fragment, variant, or derivative thereof, including but not limited to the HA, NA, NP, PA, PB1, PB2, NS1, NS2, M1 or M2 proteins or fragments (e.g., M2e), variants or derivatives thereof. In certain embodiments, a derivative protein can be a fusion protein, where the fusion protein contains a pan-DR binding epitope (e.g., M2e-PADRE®-HA). In other embodiments, the isolated influenza polypeptide or fragment, variant, or derivative thereof can be fused to a heterologous protein, e.g., a secretory signal peptide or the hepatitis B virus core protein. Preferably, the isolated influenza polypeptide or fragment, variant, or derivative thereof comprises at least one immunogenic epitope of influenza virus, wherein the antigen elicits a B-cell antibody response, a T-cell antibody response, or both. In further embodiments, the isolated influenza polypeptide or fragment, variant, or derivative thereof can be fused to an HTL epitope from an influenza virus polypeptide that is capable of eliciting an immune response.
In further embodiments, the influenza HA sequence is from an influenza strain selected from the group consisting of: Human A/Viet Nam/1203/2004 (H5N1), Human A/Hong Kong/156/97 (H5N1), Human A/Hong Kong/483/97 (H5N1), Human A/Hong Kong/1073/99 (H9N2), Avian A/Chicken/HK/G9/97 (H9N2), Swine A/Swine/Hong Kong/10/98 (H9N2), Avian A/FPV/Rostock/34 (H7N1), Avian A/Turkey/Italy/4620/99 (H7N1), Avian A/FPV/Weybridge/34 (H7N7), Human A/New Caledonia/20/99 (H1N1), Human A/Hong Kong/1/68 (H3N2), Human A/Shiga/25/97 (H3N2), Human A/Singapore/1/57 (H2N2), Human A/Leningrad/134/57 (H2N2), Human A/Ann Arbor/6/60 (H2N2), Human A/Brevig Mission/1/18 (H1N1), Swine A/Swine/Wisconsin/464/98 (H1N1), Human A/Netherlands/219/03 (H7N7) and Human A/Wyoming/3/2003 (H3N2). In certain other embodiments, the influenza virus sequence is an influenza HA sequence that encodes a polypeptide at least 90%, 95% or 100% identical to a known influenza strain. The HA sequence may be a full-length HA protein which consists essentially of the HA or extracellular (ECD) domain (HA1 and HA2), the transmembrane (TM) domain, and the cytoplasmic (CYT) domain; or a fragment of the entire HA protein which consists essentially of the HA1 domain and the HA2 domain; or a fragment of the entire HA protein which consists essentially of the HA1, HA2 and the TM domain; or a fragment of the entire HA protein which consists essentially of the CYT domain; or a fragment of the entire HA protein which consists essentially of the TM domain; or a fragment of the entire HA protein which consists essentially of the HA1 domain; or a fragment of the entire HA protein which consists essentially of the HA2 domain. The HA sequence may also include an HA1/HA2 cleavage site. The HA1/HA2 cleavage site is preferably located between the HA1 and HA2 sequences, but also can be arranged in any order relative to the other sequences of the polynucleotide or polypeptide construct.
In certain preferred embodiments, the influenza HA sequence is from a pathogenic virus strain.
Table 5 on page 151 shows an alignment of M2e sequences from representative influenza virus subtype isolates as compared to a conserved human M2e sequence that is 23 amino acids in length. Positions 10, 13, 15, 17, and 19, highlighted in grey, indicate positions where amino acid substitutions can be made. In some embodiments, the M2e sequence is selected from the M2e sequences set forth in Table 5. Table 6 on page 152 shows five pairs of sequences, the first of each pair corresponding to an M2e sequence from a representative influenza virus subtype, and the second of each pair corresponding to an M2e sequence from a representative influenza virus subtype linked to a PADRE® sequence at the N-terminus. Preferred embodiments of the invention include an M2e or PADRE®-M2e sequence selected from the group consisting of sequences set forth in Table 6. In further embodiments, the M2e sequence contains amino acid substitutions at positions 10, 13, 15, 17 and/or 19. More specifically, the amino acid substitutions correspond to the following: isoleucine at position 10 is substituted with a threonine at position 10, a glutamic acid at position 13 is substituted with glycine, a glycine at position 15 is substituted with glutamic acid, an arginine at position 17 is substituted with a lysine, and/or a glutamine at position 19 is substituted with a serine, a proline at position 9 is substituted with a leucine or histidine, an aspartic acid at position 18 is substituted with a glycine, a serine at position 20 is substituted with an aspargine, a serine at position 19 is substituted with a leucine and/or a serine at position 1 is substituted with a valine.
In addition, the invention provides consensus amino acid sequences for influenza virus polypeptides, domains, fragments, variants or derivatives thereof, including, but not limited to the HA, NA, NP, PA, PB1, PB2, NS1, NS2, M1 or M2 proteins or fragments (e.g. M2e), variants or derivatives thereof. Polynucleotides which encode the consensus polypeptides or fragments, variants or derivatives thereof, are also embodied in this invention. Such polynucleotides can be obtained by known methods, for example by backtranslation of the amino acid sequence and PCR synthesis of the corresponding polynucleotide as described below.
In addition, the influenza virus polypeptide, fragments, variants or derivatives thereof can be a fragment of a full-length influenza virus polypeptide and/or can be altered so as to, for example, remove from the polypeptide non-desired protein motifs present in the polypeptide or virulence factors associated with the polypeptide. For example, the polypeptide could be altered so as not to encode a membrane anchoring region that would prevent release of the polypeptide from the cell.
In certain embodiments, the polynucleotide of the invention comprises a spacer sequence between one and eight amino acids in length, where the spacer optimizes HTL epitope processing and minimizes junctional epitopes. In preferred embodiments, the spacer is selected from the group consisting of G, P and N, and encodes an amino acid sequence selected from the group consisting of: an amino acid sequence comprising or consisting of GPGPG (SEQ ID NO:3), an amino acid sequence comprising or consisting of PGPGP (SEQ ID NO:4), an amino acid sequence comprising or consisting of (GP)n (SEQ ID NO: 173), an amino acid sequence comprising or consisting of (PG)n (SEQ ID NO:174), an amino acid sequence comprising or consisting of (GP)nG (SEQ ID NO:175), and an amino acid sequence comprising or consisting of (PG)nP (SEQ ID NO:176), where n is an integer between zero and eleven.
In further embodiments of the present invention, the nucleic acid encoding the influenza virus HA sequence, or fragment thereof is flanked by or linked to a spacer. According to the present invention, the nucleic acid sequence encoding PADRE® epitope and/or the nucleic acid sequence encoding each HTL epitope can also be flanked by or linked to a spacer.
In further embodiments, the HTL epitope is an influenza epitope selected from the group of epitopes as set forth in Table 3. In preferred embodiments, the HTL epitope of the present invention is an influenza epitope selected from the group of epitopes as set forth in Table 4. Certain HTL epitopes in Table 4 were reevaluated for binding affinity. These results are set forth in Table 7. In additional embodiments, the HTL epitope is one derived from a non-influenza protein such as tetanus toxoid (TT), diphtheria toxoid (DT), the circumsporozoite protein of Plasmodium falciparum, the outer membrane complex of Neiserria meningitidis, Hepatitis B Surface Antigen, Hepatitis B Core Antigen, keyhole limpet hemocyanin, Rotavirus capsid protein or LI protein.
Additional polypeptides of the present invention include HA, M2e or other influenza polypeptides, or fragments, or variants thereof, interrupted by the PADRE® sequence, or having the PADRE® sequence positioned at the N-terminus or C-terminus of the polypeptide, or fragment, or variant thereof. An HA, M2e or other influenza polypeptide “interrupted” by the PADRE® sequence corresponds to a polypeptide where the PADRE® sequence is inserted at any position along the HA or other influenza polypeptide sequence, and more preferably inserted on the N- or C-terminus of an HA or other influenza polypeptide domain. For example, polypeptides of the present invention include, but are not limited to a polypeptide comprising the HA extracellular (ECD) domain and PADRE®, the HA transmembrane (TM) domain and PADRE®, or the HA cytoplasmic (CYT) domain and PADRE®, as well as polypeptides comprising HA ECD, HA TM and PADRE®; polypeptides comprising HA TM, HA CYT and PADRE®; and polypeptides comprising HA ECD, HA CYT domains and PADRE®, where the PADRE® is positioned at the N-terminus or the C-terminus of the polypeptide, or where the polypeptide is interrupted by PADRE® sequence. Additional polynucleotides of the present invention include nucleic acid sequences encoding the polypeptides set forth above.
A further example of a polypeptide of the present invention is a polypeptide comprising an HA, M2e or influenza polypeptide, or fragment, variant or derivative thereof, as set further above and optionally one to ten polypeptides consisting of an HTL epitope. The one or more HTL epitopes of the present invention may be positioned at the N-terminus or C-terminus of the HA, M2e or influenza polypeptide, or fragment, variant, or derivative thereof. Representative influenza HTL epitopes according to the invention can found at Table 3. Preferred influenza HTL epitopes of the present invention can be found at Table 4. HTL epitopes selected from Table 4 that were reevaluated for binding as shown in Table 7 are also epitopes of the present invention. Additional polynucleotides of the present invention include nucleic acid sequences encoding the polypeptides set forth above.
In certain embodiments, the polynucleotide further comprises a nucleic acid encoding a targeting sequence located at the N-terminus of said construct. In further embodiments, the targeting sequence is selected from the group consisting of: an Ig kappa signal sequence, a tissue plasminogen activator signal sequence, an insulin signal sequence, an endoplasmic reticulum signal sequence, a LAMP-1 lysosomal targeting sequence, a LAMP-2 lysosomal targeting sequence, an HLA-DM lysosomal targeting sequence, an HLA-DM-association sequence of HLA-DO, an Ig-a cytoplasmic domain, Ig-ss cytoplasmic domain, a li protein, an influenza matrix protein, an HCV antigen, and a yeast Ty protein, a baculovirus signal sequence, a BiP signal sequence, a chitinase signal sequence or a prokaryotic signal sequence. In a preferred embodiment a chitinase or a BiP signal sequence are at the N-terminus of the construct. However, the chitinase and/or BiP can also be at the C-terminus or arranged in any order relative to the other sequences of the polynucleotide or polypeptide construct.
In certain embodiments, the polynucleotide further comprises a thrombin cleavage site and/or a trimerization sequence. In particular, the trimerization sequence may be a “foldon” sequence. According to the present invention, the polynucleotide can comprise a thrombin and a foldon sequence located at the C-terminus of said construct. The invention also contemplates the use of a thrombin cleavage and/or foldon sequence arranged in any order relative to the other sequences of the polynucleotide or polypeptide sequence. In one preferred embodiment, the thrombin cleavage site is located between the foldon sequence and the PADRE®-HA or HA sequence.
In a preferred embodiment of the invention, the polynucleotide includes a chitinase signal sequence, a HIS tag, optionally a PADRE® sequence and an HA sequence. The HA sequence can include a wild-type or mutant HA1/HA2 cleavage site and/or the membrane and/or cytoplasmic HA domains.
In another preferred embodiment, the polynucleotide includes a Bip signal sequence, a HIS tag, optionally a PADRE® sequence, an HA sequence, a thrombin cleavage signal, and a foldon sequence. The HA sequence can include a wild-type or a mutant HA1/HA2 cleavage site.
Nucleic acids and fragments thereof of the present invention can be altered from their native state in one or more of the following ways. First, a nucleic acid or fragment thereof which encodes an influenza virus polypeptide can be a fragment which encodes only a portion of a full-length polypeptide, and/or can be mutated so as to, for example, remove from the encoded polypeptide non-desired protein motifs present in the encoded polypeptide or virulence factors associated with the encoded polypeptide. For example, the nucleic acid sequence could be mutated so as not to encode a membrane anchoring region that would prevent release of the polypeptide from the cell as with, e.g., M2e. Upon delivery, the polynucleotide of the invention is incorporated into the cells of the vertebrate in vivo, and a prophylactically or therapeutically effective amount of an immunologic epitope of an influenza virus is produced in vivo. Alternatively, epitopes may be modified (to create analogs thereof) to increase their immunogenicity as compared to native epitopes.
The present invention further provides polypeptides encoded by the polynucleotides described above, a vector comprising the polynucleotides described above as well as immunogenic compositions comprising the polynucleotides and/or polypeptides described above. In certain other embodiments, the present invention is directed to a cell comprising polynucleotides, polypeptides, or immunogenic compositions as described above. In certain other embodiments, a composition comprises two or more polypeptides as described above, where the polypeptides are different from each other.
In certain other embodiments, the invention provides immunogenic compositions comprising at least one polynucleotide of the present invention, or a polypeptide encoded by at least one polynucleotide of the present invention, where the polynucleotide comprises a nucleic acid sequence of a coding region operably encoding an influenza virus polypeptide, fragment, variant, or derivative thereof and a pan-DR binding epitope (e.g. PADRE®) and/or one or more nucleic acids encoding a helper T lymphocyte (HTL) epitope. Such compositions can further comprise, for example, carriers, excipients, transfection facilitating agents, lipids, liposomes, virosomes and/or adjuvants as described herein.
In certain embodiments, immunogenic compositions can further comprise, for example, carriers, excipients, transfection facilitating agents, lipids, liposomes and/or adjuvants as described herein. In certain other embodiments, immunogenic compositions can further comprise a virosome. For example, the PADRE®-HA protein may be inserted into a virosome lipid bilayer. In further embodiments, the virosome is an immunopotentiating reconstituted influenza virosome (IRIV).
The compositions of the invention can be univalent, bivalent, trivalent or multivalent. A univalent composition will comprise only one polynucleotide of the present invention, or a polypeptide encoding the polynucleotide of the present invention, where the polynucleotide comprises a nucleic acid sequence of a coding region encoding an influenza virus polypeptide or a fragment, variant, or derivative thereof, a PADRE® epitope and, optionally, an HTL epitope and/or a second influenza virus polypeptide or a fragment, variant, or derivative thereof. A bivalent composition will comprise, either in polynucleotide or polypeptide form, two different influenza virus polypeptides, fragments, variants, or derivatives thereof, each capable of eliciting an immune response. The polynucleotide(s) of the composition can encode two influenza virus polypeptides or alternatively, the polynucleotide can encode only one influenza virus polypeptide and the second influenza virus polypeptide would be provided by an isolated influenza virus polypeptide of the invention as in, for example, a single formulation heterologous prime-boost vaccine composition. In the case where both influenza virus polypeptides of a bivalent composition are delivered in polynucleotide form, the nucleic acid fragments operably encoding those influenza virus polypeptides need not be on the same polynucleotide, but can be on two different polynucleotides. A trivalent or further multivalent composition will comprise three influenza virus polypeptides or fragments, variants or derivatives thereof, either in isolated form or encoded by one or more polynucleotides of the invention.
The present invention further provides plasmids and other polynucleotide constructs for delivery of nucleic acid fragments of the invention to a vertebrate, e.g., a human, which provide expression of influenza virus polypeptides, or fragments, variants, or derivatives thereof. The present invention further provides carriers, excipients, transfection-facilitating agents, immunogenicity-enhancing agents, e.g., adjuvants, or other agent or agents to enhance the transfection, expression or efficacy of the administered gene and its gene product.
In one embodiment, a multivalent composition comprises a single polynucleotide, e.g., plasmid, comprising one or more nucleic acid regions operably encoding influenza polypeptides or fragments, variants, or derivatives thereof. Reducing the number of polynucleotides, e.g., plasmids, in the compositions of the invention can have significant impacts on the manufacture and release of product, thereby reducing the costs associated with manufacturing the compositions. There are a number of approaches to include more than one expressed antigen coding sequence on a single plasmid. These include, for example, the use of Internal Ribosome Entry Site (IRES) sequences, dual promoters/expression cassettes, and fusion proteins.
The present invention is further directed to enhancing the immune response of a vertebrate in need of protection against influenza virus infection by administering, in vivo, into a tissue of the vertebrate, a polynucleotide, a polypeptide, or a composition as described above. The isolated polypeptide can be, for example, a purified subunit, a recombinant protein, a viral vector expressing an isolated influenza virus polypeptide, or can be an inactivated or attenuated influenza virus, such as those present in conventional influenza virus vaccines. According to either method, the polynucleotide is incorporated into the cells of the vertebrate in vivo, and an immunologically effective amount of an immunogenic epitope of the encoded influenza virus polypeptide, or a fragment, variant, or derivative thereof, is produced in vivo. When utilized, an isolated influenza virus polypeptide or a fragment, variant, or derivative thereof is also administered in an immunologically effective amount.
The invention also provides methods for enhancing the immune response of a vertebrate to influenza virus infection by administering to the tissues of a vertebrate one or more polypeptides, domains, fragments, or variants thereof of the present invention or one or more polynucleotides encoding one or more polypeptides, domains, fragments, or variants thereof of the present invention.
FIGS. 2A-D. PADRE® increases HA-Specific Antibody Responses in Individual Animals. Results of antibody titer levels in individual animals immunized with 100 μg or 1 μg of HA or PADRE®-HA. Immunization of animals and subsequent measurements of HA-specific antibody titers using enzyme-linked immunosorbent assays were performed as described above.
FIGS. 3A-B. HTL Human Recall Responses in Donor X753. Immune responses in Donor X753 using a panel of negative control HTL epitope-containing peptides and a panel of HTL epitope-containing peptides derived from internal flu proteins, NS1, NS2, PB1, PB2, PA, NP, M1 and M2. Assays were performed as described in Example 6 below. The sequences of the HTL epitopes used in the experiment correspond to the nomenclature of the influenza HTL candidates in Tables 3 and 4.
FIGS. 4A-B. Immune Human Recall Responses in Donor 753. Immune responses in Donor 753 using a panel of negative control peptides derived from HIV and HCV and a panel of peptides derived from influenza. Data are shown as spot forming cells/million CD4+ PBMC. Assays were performed as described in Example 6 below. The sequences of the influenza peptides used in the experiment correspond to the nomenclature in Tables 3-4 and 7.
FIGS. 5A-B. Immune Human Recall Responses in Donor 6018. Immune responses in Donor 6018 using a panel of negative control peptides derived from HIV and HCV and a panel of peptides derived from influenza. Data are shown as spot forming cells/million CD4+ PBMC. Assays were performed as described in Example 6 below. The sequences of the influenza peptides used in the experiment correspond to the nomenclature in Tables 3-4 and 7.
FIGS. 6A-B Immune Human Recall Responses in Donor 716. Immune responses in Donor 716 using a panel of negative control peptides derived from HIV and HCV and a panel of peptides derived from influenza. Data are shown as spot forming cells/million CD4+ PBMC. Assays were performed as described in Example 6 below. The sequences of the influenza peptides used in the experiment correspond to the nomenclature in Tables 3-4 and 7.
FIGS. 7A-B. Immune Human Recall Responses in Donor AC08. Immune responses in Donor AC08 using a panel of negative control peptides derived from HIV and HCV and a panel of peptides derived from influenza. Data are shown as spot forming cells/million CD4+ PBMC. Assays were performed as described in Example 6 below. The sequences of the influenza peptides used in the experiment correspond to the nomenclature in Tables 3-4 and 7.
FIGS. 8A-B. Immune Human Recall Responses in Donor AC02. Immune responses in Donor AC02 using a panel of negative control peptides derived from HIV and HCV and a panel of peptides derived from influenza. Data are shown as spot forming cells/million CD4+ PBMC. Assays were performed as described in Example 6 below. The sequences of the influenza peptides used in the experiment correspond to the nomenclature in Tables 3-4 and 7.
FIGS. 9A-B. Immune Human Recall Responses in Donor 3501. Immune responses in Donor 3501 using a panel of negative control peptides derived from HIV and HCV and a panel of peptides derived from influenza. Data are shown as spot forming cells/million CD4+ PBMC. Assays were performed as described in Example 6 below. The sequences of the influenza peptides used in the experiment correspond to the nomenclature in Tables 3-4 and 7.
The present invention is directed to compositions and methods for enhancing the immune response of a vertebrate in need of protection against influenza virus infection by administering in vivo, into a tissue of a vertebrate, at least one polynucleotide or at least one polypeptide encoded by such a polynucleotide, comprising or encoded by one or more nucleic acid fragments, where each nucleic acid fragment is a fragment of a coding region operably encoding an influenza virus polypeptide, or a fragment, variant, or derivative thereof in cells of the vertebrate in need of protection. The polynucleotide or polypeptide also comprises a nucleic acid sequence encoding a pan-DR binding epitope (e.g. PADRE®) or the peptide encoded therein and optionally one or more nucleic acids encoding a sequence that comprises a helper T lymphocyte (HTL) epitope or the polypeptide encoded therein.
The present invention is also directed to administering in vivo, into a tissue of the vertebrate the above described polynucleotide and at least one isolated influenza polypeptide, or a fragment, variant, or derivative thereof. The isolated influenza polypeptide or fragment, variant, or derivative thereof can be, for example, a recombinant protein, a purified subunit protein, a protein expressed and carried by a heterologous live or inactivated or attenuated viral vector expressing the protein, or can be an inactivated influenza, such as those present in conventional, commercially available, inactivated influenza vaccines. According to either method, the polynucleotide is incorporated into the cells of the vertebrate in vivo, and an immunologically effective amount of the influenza protein, or fragment or variant encoded by the polynucleotide is produced in vivo. The isolated protein or fragment, variant, or derivative thereof is also administered in an immunologically effective amount. The polynucleotide can be administered to the vertebrate in need thereof either prior to, at the same time (simultaneously), or subsequent to the administration of the isolated influenza polypeptide or fragment, variant, or derivative thereof.
Non-limiting examples of influenza polypeptides within the scope of the invention include, but are not limited to, HA, NA, NP, PA, PB1, PB2, NS1, NS2, M1 or M2 polypeptides, and fragments, e.g., M2e derivatives, and variants thereof. Nucleotide and amino acid sequences of influenza polypeptides from a wide variety of influenza types and subtypes are known in the art. The nucleotide sequences and polypeptide sequences set forth below comprise wild-type HA sequences. For example, the amino acid sequence corresponding to the mature HA protein of Influenza A/Vietnam/1203/2004 (H5N1) is available in GenBank (Accession Number AAT73274), and has the following sequence, referred to herein as SEQ ID NO: 5:
Polypeptides of the present invention also include the extracellular domain (ECD) of the HA protein, for example, of Influenza A/Vietnam/1203/2004 (H5N1), having the following sequence, referred to herein as SEQ ID NO: 6:
Polypeptides of the present invention may further include the transmembrane domain (TM) of the HA protein, for example, of Influenza A/Vietnam/1203/2004 (H5N1) having the sequence ILSIYSTVASSLALAIMVAGL (SEQ ID NO: 7) and/or the cytoplasmic domain (CYT) of the HA protein, for example, of Influenza A/Vietnam/1203/2004 (H5N1) having the sequence SLWMCSNGSLQCR (SEQ ID NO:8).
Additional HA sequences of the present invention correspond to isolated wild-type HA sequences from influenza A and influenza B strains as disclosed in Tables 1 and 2. Wild-type HA sequences from influenza strains can also be found at http://www.flu.lanl.gov/search/index.html?form_page=search.
Additional polypeptides of the present invention include polypeptides comprising the ECD domain, the TM domain, or the CYT domain of the HA sequences set forth above, and any combinations thereof, including, but not limited to HA polypeptides comprising the ECD, TM and CYT domains; polypeptides comprising both the ECD and TM domains; polypeptides comprising both the TM and CYT domains; and polypeptides comprising the ECD and CYT domains. Polypeptides of the present invention can optionally comprise a N-terminal sequence, for example, residues 1-16 of the HA sequence available in Genbank (Accession Number AAT73274), which corresponds to the natural signal sequence and/or other appropriate signal sequences known in the art.
Polynucleotides of the present invention can comprise a heterologous signal sequence, a His-tag sequence, a wild-type HA sequence and/or a PADRE® sequence. For example, the polynucleotide sequence of an exemplary HA construct comprising a heterologous signal sequence, a His-tag sequence, and a wild-type HA sequence of the present invention is as follows, referred to herein as SEQ ID NO: 9:
The amino acid sequence of this exemplary HA construct described above is as follows (highlighted portion corresponds to heterologous signal sequence and His-tag sequence), referred to herein as SEQ ID NO:10:
The amino acid sequence of this exemplary HA-PADRE® construct described above is as follows (highlighted portion corresponds to heterologous signal sequence and His-tag sequence; underlined portion corresponds to PADRE® sequence), referred to herein as SEQ ID NO:12:
The polynucleotide sequence of an exemplary PADRE®-HA construct of the present invention is as follows, referred to herein as SEQ ID NO: 13:
The amino acid sequence of this exemplary PADRE®-HA construct described above is as follows (highlighted portion corresponds to heterologous signal sequence and His-tag sequence; underlined portion corresponds to PADRE® sequence), referred to herein as SEQ ID NO:14:
Polynucleotides of the present invention can also comprise a HIS tag. The HIS tag can be a 6×HIS tag of the sequence or can be a HIS tag of the sequence MKHQHQHQHQHQHQ (SEQ ID NO: 176). The HIS tag can optionally be followed or proceeded by a sequence to allow for removal of the HIS tag. The sequence may, for example be a stop signal that follows the HIS tag and includes a basic amino acid in the first position adjacent to the HIS tag or a proline at the second or third position after the HIS tag. In particular, the stop sequence may be a dipeptidase stop signal of the sequence AP, GPG or GPGPG (SEQ ID NO:3). The dipeptidase stop signal may allow for removal of the HIS tag by a dipeptidase. The HIS tag also can optionally be adjacent to a TEV protease cleavage site. In a preferred embodiment the sequence that allows for removal of the HIS tag is located between the PADRE®-HA or HA sequence and the HIS tag. The HIS tag is preferably located on the N-terminus of the PADRE®-HA or HA sequence, but can be arranged in any order relative to the other sequences.
Polynucleotides of the present invention also can include a cleavage site. Optionally, the cleavage site can be located between the HA1 and HA1 sequences. The cleavage site can be, for example the endogenous cleavage site of H5 of A/Vietnam/1203/2004 HA polybasic cleavage site PQRERRRKKRGLFGAI (SEQ ID NO: 186), which is expected to be cleaved during secretion. The cleavage site can also be a mutated version of the cleavage site with the sequence PQRETQGLFGAI (SEQ ID NO:187), which is not expected to be cleaved. The cleavage site can also be a thrombin cleavage site, for example, of the sequence, SSGRLVPRGSPGS (SEQ ID NO:178). The cleavage site can also be a TEV protease cleavage site, for example, of the sequence DYDIPTTENLYFQGA (SEQ ID NO: 188).
Polynucleotides of the present invention can also include a trimerizing sequence. Influenza HA is expressed as a trimeric membrane bound protein with a C-terminal cytosolic tail. In general, proteins embedded in the membrane are more difficult to purify and are expressed in much less quantities compared to proteins that are secreted as soluble proteins. Therefore, some constructs of the present invention are designed to encode only the HA ectodomain (without membrane and cytoplasmic regions) to allow for efficient secretion of the recombinant protein. However, as the trimeric structure of HA is important for its antigenicity, a trimerizing sequence (‘foldon’) from the bacteriophage T4 fibritin can be added in place of the transmembrane and cytoplasmic domains. The fold-on sequence has been shown to facilitate the trimerization of influenza HA155-156 as well as collagen. The fold-on may enhance formation of a stable trimer to ensure that antibodies raised against the recombinant truncated protein crossreact with the native HA.
Polynucleotides of the present invention can comprise a signal sequence, a HIS-tag sequence and optionally a TEV protease cleavage site, optionally a PADRE® sequence, an HA1 sequence, an HA1/HA2 cleavage site, an HA2 sequence, an HA transmembrane sequence and an HA cytoplasmic domain. For example, an exemplary example of such a polynucleotide that includes a PADRE® sequence is as follows, referred to herein as SEQ ID NO:182:
The amino acid sequence of this exemplary construct described above is as follows, referred to herein as SEQ ID NO: 183 (in which aa 1-24 correspond to a chitinase signal sequence, aa 25-30 correspond to a 6×HIS tag, aa 31-45 correspond to a TEV protease cleavage site, aa 46-58 correspond to PADRE® and aa 59-607 correspond to A/Vietnam/1203/2004 HA seq (Acc #AAT73274),
An exemplary example of such a polynucleotide that does not include a PADRE sequence is as follows, referred to herein as SEQ ID NO: 180:
The amino acid sequence of this exemplary construct described above is as follows, referred to herein as SEQ ID NO: 181 (in which aa 1-24 correspond to a chitinase signal sequence, aa 25-30 correspond to a 6×HIS tag, aa 31-45 correspond to a TEV protease cleavage site and aa 46-594 correspond to A/Vietnam/1203/2004 HA seq (Acc #AAT73274).
Polynucleotides of the present invention can comprise a signal sequence, a HIS-tag sequence, optionally a PADRE® sequence, an HA1 sequence, an HA1/HA2 cleavage site, an HA2 sequence, thrombin cleavage site and a foldon sequence. For example, an exemplary example of such a polynucleotide that includes a PADRE® sequence is as follows, referred to herein as SEQ ID NO:173:
The amino acid sequence of this exemplary construct described above is as follows, referred to herein as SEQ ID NO:174 (in which aa 1-18 correspond to a Bip signal sequence, aa 19-32 correspond to a HIS tag, aa 33-34 correspond to a dipeptidase stop signal, aa 35-47 correspond to PADRE®, aa 552-563 correspond to a thrombin cleavage site and aa 564-590 correspond to a foldon sequence.
An exemplary example of such a polynucleotide that does not include a PADRE® sequence is as follows, referred to herein as SEQ ID NO: 184:
The amino acid sequence of this exemplary construct described above is as follows, referred to herein as SEQ ID NO:185 (in which aa 1-18 correspond to a BiP signal sequence, aa 19-32 correspond to a HIS tag, aa 33-34 correspond to a dipeptidase stop signal, aa 539-550 correspond to a thrombin cleavage site and aa 551-577 correspond to a foldon sequence.
In certain embodiments, the M2e polypeptides for use in the present invention correspond to the M2e polypeptides set forth in Table 5. Preferred M2e and PADRES M2e polypeptides of the present invention are set forth in Table 6.
In certain other embodiments, polypeptides of the present invention include SEQ ID NOs: 174, 181, 183 and 185.
In certain embodiments, the polynucleotide of the invention comprises a nucleic acid encoding from about zero to about ten HTL epitopes. In other embodiments, the polypeptide of the invention comprises from about zero to about ten HTL epitopes. The term “HTL epitope” refers to a peptide of defined length that can be from about 6 to about 30 amino acids in length, from about 8 to about 30 amino acids in length, from about 10 to about 30 amino acids, from about 12 to about 30 amino acids in length, from about 6 to about 25 amino acids in length, from about 8 to about 25 amino acids in length, from about 10 to about 25 amino acids, from about 12 to about 25 amino acids in length, from about 6 to about 18 amino acids in length, from about 8 to about 18 amino acids in length, from about 10 to about 18 amino acids, or from about 12 to about 18 amino acids in length, which is recognized by a particular HLA molecule. The one to ten HTL epitopes of the present invention are positioned at the N-terminus or C-terminus of the HA, M2e or influenza polypeptide, or fragment, variant, or derivative thereof. Representative influenza HTL epitopes according to the invention can found at Table 3. Preferred influenza HTL epitopes of the present invention can be found at Table 4. Certain HTL epitopes in Table 4 were reevaluated for binding affinity. These results are set forth in Table 7. Additional polynucleotides of the present invention include nucleic acid sequences encoding the polypeptides set forth above.
Additional polypeptides of the present invention further include HA, M2e or other influenza polypeptides, or fragment, variant or derivatives thereof, interrupted by a pan-DR binding epitope, preferably the PADRE® sequence, or having the pan-DR binding epitope or PADRE® sequence positioned at the N-terminus or C-terminus of the polypeptide, or fragment, variant, or derivative thereof. An HA, M2e or other influenza polypeptide “interrupted” by the pan-DR binding epitope or PADRE® sequence corresponds to a polypeptide where the pan-DR binding epitope or PADRE® sequence is inserted at any position along the HA or other influenza polypeptide sequence, and more preferably inserted at the N- or C-terminus of an HA or other influenza polypeptide domain. An insertion may leave the rest of the influenza polypeptide intact, or may replace a segment of the influenza polypeptide. For example, polypeptides of the present invention include, but are not limited to a polypeptide comprising HA ECD and PADRE®; HA TM and PADRE®; or HA CYT and PADRE®. Further polypeptides of the invention include polypeptides comprising HA ECD, HA TM and PADRE®; polypeptides comprising HA TM, HA CYT and PADRE®; and polypeptides comprising HA ECD, HA CYT and PADRE®; where the PADRE® is positioned at the N-terminus or the C-terminus of the polypeptide, or where the polypeptide is interrupted by PADRE® sequence. Additional polynucleotides of the present invention include nucleic acid sequences encoding the polypeptides set forth above.
A further example of a polypeptide of the present invention is a polypeptide comprising an HA, M2e or influenza polypeptide, or fragment, variant or derivative thereof, as set further above and optionally one to ten polypeptides each consisting of an HTL epitope.
Methods of designing and selecting HTL epitopes having an HLA-DR binding motif according to the present invention are described in Rammensee et al., “MHC ligands and peptide motifs: first listing,” Immunogenetics 41:178-228 (1995) and Sette et al., “Prediction of major histocompatibility complex binding regions of protein antigens by sequence pattern analysis,” Proc. Natl. Acad. Sci. 86: 3296-3300 (1989), the disclosure of each which is incorporated herein by reference in its entirety.
Methods of designing and generating a multi-epitope construct comprising an HA, M2e or influenza polypeptide, or fragment, variant or derivative thereof, and/or one or more HTL epitopes are performed according to methods of designing and using multi-epitope constructs as described in WO 01/47541 and WO 02/083714, the disclosure of each which is incorporated herein by reference in its entirety.
The present invention also provides vaccine compositions and methods for delivery of influenza virus coding sequences to a vertebrate with optimal expression and safety. These vaccine compositions are prepared and administered in such a manner that the encoded gene products are optimally expressed in the vertebrate of interest. As a result, these compositions and methods are useful in stimulating an immune response against influenza virus infection. Also included in the invention are expression systems and delivery systems.
It is to be noted that the term “a” or “an” entity refers to one or more of that entity; for example, “a polynucleotide,” is understood to represent one or more polynucleotides. As such, the terms “a” (or “an”), “one or more,” and “at least one” can be used interchangeably herein.
The term “polynucleotide” is intended to encompass a singular nucleic acid or nucleic acid fragment as well as plural nucleic acids or nucleic acid fragments, and refers to an isolated molecule or construct, e.g., a virus genome (e.g., a non-infectious viral genome), messenger RNA (mRNA), plasmid DNA (pDNA), or derivatives of pDNA (e.g., minicircles as described in (Darquet, A-M et al., Gene Therapy 4:1341-1349 (1997)) comprising a polynucleotide. A polynucleotide may comprise a conventional phosphodiester bond or a non-conventional bond (e.g., an amide bond, such as found in peptide nucleic acids (PNA)).
The terms “nucleic acid” or “nucleic acid fragment” refer to any one or more nucleic acid segments, e.g., DNA or RNA fragments, present in a polynucleotide or construct. A nucleic acid or fragment thereof may be provided in linear (e.g., mRNA) or circular (e.g., plasmid) form as well as double-stranded or single-stranded forms. By “isolated” nucleic acid or polynucleotide is intended a nucleic acid molecule, DNA or RNA, which has been removed from its native environment. For example, a recombinant polynucleotide contained in a vector is considered isolated for the purposes of the present invention. Further examples of an isolated polynucleotide include recombinant polynucleotides maintained in heterologous host cells or purified (partially or substantially) polynucleotides in solution. Isolated RNA molecules include in vivo or in vitro RNA transcripts of the polynucleotides of the present invention. Isolated polynucleotides or nucleic acids according to the present invention further include such molecules produced synthetically.
As used herein, a “coding region” is a portion of nucleic acid which consists of codons translated into amino acids. Although a “stop codon” (TAG, TGA, or TAA) is not translated into an amino acid, it may be considered to be part of a coding region, but any flanking sequences, for example promoters, ribosome binding sites, transcriptional terminators, and the like, are not part of a coding region. Two or more nucleic acids or nucleic acid fragments of the present invention can be present in a single polynucleotide construct, e.g., on a single plasmid, or in separate polynucleotide constructs, e.g., on separate (different) plasmids. Furthermore, any nucleic acid or nucleic acid fragment may encode a single influenza polypeptide or fragment, derivative, or variant thereof, e.g., or may encode more than one polypeptide, e.g., a nucleic acid may encode two or more polypeptides. In addition, a nucleic acid may include a regulatory element such as a promoter, ribosome binding site, or a transcription terminator, or may encode heterologous coding regions fused to the influenza coding region, e.g., specialized elements or motifs, such as a secretory signal peptide or a heterologous functional domain.
The terms “fragment,” “variant,” “derivative” and “analog” when referring to influenza virus polypeptides of the present invention include any polypeptides which retain at least some of the immunogenicity or antigenicity of the corresponding native polypeptide. Fragments of influenza virus polypeptides of the present invention include proteolytic fragments, deletion fragments and in particular, fragments of influenza virus polypeptides which exhibit increased secretion from the cell or higher immunogenicity or reduced pathogenicity when delivered to an animal, such as deletion of signal sequences or one or more domains. Polypeptide fragments further include any portion of the polypeptide which comprises an antigenic or immunogenic epitope of the native polypeptide, including linear as well as three-dimensional epitopes. Variants of influenza virus polypeptides of the present invention include fragments as described above, and also polypeptides with altered amino acid sequences due to amino acid substitutions, deletions, or insertions. Variants may occur naturally, such as an allelic variant. By an “allelic variant” is intended alternate forms of a gene occupying a given locus on a chromosome or genome of an organism or virus. Genes II, Lewin, B., ed., John Wiley & Sons, New York (1985), which is incorporated herein by reference. For example, as used herein, variations in a given gene product. When referring to influenza virus NA or HA proteins, each such protein is a “variant,” in that native influenza virus strains are distinguished by the type of NA and HA proteins encoded by the virus. However, within a single HA or NA variant type, further naturally or non-naturally occurring variations such as amino acid deletions, insertions or substitutions may occur. Non-naturally occurring variants may be produced using art-known mutagenesis techniques. Variant polypeptides may comprise conservative or non-conservative amino acid substitutions, deletions or additions. Derivatives of influenza virus polypeptides of the present invention are polypeptides which have been altered so as to exhibit additional features not found on the native polypeptide. Examples include fusion proteins. An analog is another form of an influenza virus polypeptide of the present invention. An example is a proprotein which can be activated by cleavage of the proprotein to produce an active mature polypeptide.
The terms “infectious polynucleotide” or “infectious nucleic acid” are intended to encompass isolated viral polynucleotides and/or nucleic acids which are solely sufficient to mediate the synthesis of complete infectious virus particles upon uptake by permissive cells. Thus, “infectious nucleic acids” do not require pre-synthesized copies of any of the polypeptides it encodes, e.g., viral replicases, in order to initiate its replication cycle in a permissive host cell.
The terms “non-infectious polynucleotide” or “non-infectious nucleic acid” as defined herein are polynucleotides or nucleic acids which cannot, without additional added materials, e.g., polypeptides, mediate the synthesis of complete infectious virus particles upon uptake by permissive cells. An infectious polynucleotide or nucleic acid is not made “non-infectious” simply because it is taken up by a non-permissive cell. For example, an infectious viral polynucleotide from a virus with limited host range is infectious if it is capable of mediating the synthesis of complete infectious virus particles when taken up by cells derived from a permissive host (i.e., a host permissive for the virus itself). The fact that uptake by cells derived from a non-permissive host does not result in the synthesis of complete infectious virus particles does not make the nucleic acid “non-infectious.” In other words, the term is not qualified by the nature of the host cell, the tissue type, or the species taking up the polynucleotide or nucleic acid fragment.
In some cases, an isolated infectious polynucleotide or nucleic acid may produce fully-infectious virus particles in a host cell population which lacks receptors for the virus particles, i.e., is non-permissive for virus entry. Thus viruses produced will not infect surrounding cells. However, if the supernatant containing the virus particles is transferred to cells which are permissive for the virus, infection will take place.
The terms “replicating polynucleotide” or “replicating nucleic acid” are meant to encompass those polynucleotides and/or nucleic acids which, upon being taken up by a permissive host cell, are capable of producing multiple, e.g., one or more copies of the same polynucleotide or nucleic acid. Infectious polynucleotides and nucleic acids are a subset of replicating polynucleotides and nucleic acids; the terms are not synonymous. For example, a defective virus genome lacking the genes for virus coat proteins may replicate, e.g., produce multiple copies of itself, but is NOT infectious because it is incapable of mediating the synthesis of complete infectious virus particles unless the coat proteins, or another nucleic acid encoding the coat proteins, are exogenously provided.
In certain embodiments, the polynucleotide, nucleic acid, or nucleic acid fragment is DNA. In the case of DNA, a polynucleotide comprising a nucleic acid which encodes a polypeptide normally also comprises a promoter and/or other transcription or translation control elements operably associated with the polypeptide-encoding nucleic acid fragment. An operable association is when a nucleic acid fragment encoding a gene product, e.g., a polypeptide, is associated with one or more regulatory sequences in such a way as to place expression of the gene product under the influence or control of the regulatory sequence(s). Two DNA fragments (such as a polypeptide-encoding nucleic acid fragment and a promoter associated with the 5′ end of the nucleic acid fragment) are “operably associated” if induction of promoter function results in the transcription of mRNA encoding the desired gene product and if the nature of the linkage between the two DNA fragments does not (1) result in the introduction of a frame-shift mutation, (2) interfere with the ability of the expression regulatory sequences to direct the expression of the gene product, or (3) interfere with the ability of the DNA template to be transcribed. Thus, a promoter region would be operably associated with a nucleic acid fragment encoding a polypeptide if the promoter was capable of effecting transcription of that nucleic acid fragment. The promoter may be a cell-specific promoter that directs substantial transcription of the DNA only in predetermined cells. Other transcription control elements, besides a promoter, for example enhancers, operators, repressors, and transcription termination signals, can be operably associated with the polynucleotide to direct cell-specific transcription. Suitable promoters and other transcription control regions are disclosed herein.
A variety of transcription control regions are known to those skilled in the art. These include, without limitation, transcription control regions which function in vertebrate cells, such as, but not limited to, promoter and enhancer segments from cytomegaloviruses (the immediate early promoter, in conjunction with intron-A), simian virus 40 (the early promoter), and retroviruses (such as Rous sarcoma virus). Other transcription control regions include those derived from vertebrate genes such as actin, heat shock protein, bovine growth hormone and rabbit 3-globin, as well as other sequences capable of controlling gene expression in eukaryotic cells. Additional suitable transcription control regions include tissue-specific promoters and enhancers as well as lymphokine-inducible promoters (e.g., promoters inducible by interferons or interleukins).
Similarly, a variety of translation control elements are known to those of ordinary skill in the art. These include, but are not limited to ribosome binding sites, translation initiation and termination codons, elements from picornaviruses (particularly an internal ribosome entry site, or IRES, also referred to as a CITE sequence).
A DNA polynucleotide of the present invention may be a circular or linearized plasmid or vector, or other linear DNA which may also be non-infectious and nonintegrating (i.e., does not integrate into the genome of vertebrate cells). A linearized plasmid is a plasmid that was previously circular but has been linearized, for example, by digestion with a restriction endonuclease. Linear DNA may be advantageous in certain situations as discussed, e.g., in Cherng, J. Y., et al., J. Control. Release 60:343-53 (1999), and Chen, Z. Y., et al. Mol. Ther. 3:403-10 (2001), both of which are incorporated herein by reference. As used herein, the terms plasmid and vector can be used interchangeably.
Alternatively, DNA virus genomes may be used to administer DNA polynucleotides into vertebrate cells. In certain embodiments, a DNA virus genome of the present invention is nonreplicative, noninfectious, and/or nonintegrating. Suitable DNA virus genomes include without limitation, herpesvirus genomes, adenovirus genomes, adeno-associated virus genomes, and poxvirus genomes. References citing methods for the in vivo introduction of non-infectious virus genomes to vertebrate tissues are well known to those of ordinary skill in the art, and are cited supra.
In other embodiments, a polynucleotide of the present invention is RNA, for example, in the form of messenger RNA (mRNA). Methods for introducing RNA sequences into vertebrate cells are described in U.S. Pat. No. 5,580,859, the disclosure of which is incorporated herein by reference in its entirety.
Polynucleotides, nucleic acids, and nucleic acid fragments of the present invention may be associated with additional nucleic acids which encode secretory or signal peptides, which direct the secretion of a polypeptide encoded by a nucleic acid fragment or polynucleotide of the present invention. According to the signal hypothesis, proteins secreted by mammalian cells have a signal peptide or secretory leader sequence which is cleaved from the mature protein once export of the growing protein chain across the rough endoplasmic reticulum has been initiated. Those of ordinary skill in the art are aware that polypeptides secreted by vertebrate cells generally have a signal peptide fused to the N-terminus of the polypeptide, which is cleaved from the complete or “full length” polypeptide to produce a secreted or “mature” form of the polypeptide. In certain embodiments, the native leader sequence is used, or a functional derivative of that sequence that retains the ability to direct the secretion of the polypeptide that is operably associated with it. Alternatively, a heterologous mammalian leader sequence, or a functional derivative thereof, may be used. For example, the wild-type leader sequence may be substituted with the leader sequence of human tissue plasminogen activator (TPA) or mouse β-glucuronidase.
In accordance with one aspect of the present invention, there is provided a polynucleotide construct, for example, a plasmid, comprising a nucleic acid fragment, where the nucleic acid fragment is a fragment of a coding region operably encoding an influenza virus-derived polypeptide, where the coding region is optimized for expression in vertebrate cells, of a desired vertebrate species, e.g., humans, to be delivered to a vertebrate to be treated or immunized. Suitable influenza polypeptides, or fragments, variants, or derivatives thereof may be derived from, but are not limited to, the influenza virus HA, NA, NP, PA, PB1, PB2, NS1, NS2, M1 or M2 proteins. Additional influenza-derived coding sequences, e.g., coding for HA, NA, NP, PA, PB1, PB2, NS1, NS2, M1, M2 or M2e, may also be included on the plasmid, or on a separate plasmid, and expressed, either using native influenza virus codons or codons for expression in the vertebrate to be treated or immunized. When such a plasmid encoding one or more influenza sequences is delivered, in vivo to a tissue of the vertebrate to be treated or immunized, one or more of the encoded gene products will be expressed, i.e., transcribed and translated. The level of expression of the gene product(s) will depend to a significant extent on the strength of the associated promoter and the presence and activation of an associated enhancer element, as well as the degree of optimization of the coding region.
As used herein, the term “plasmid” refers to a construct made up of genetic material (i.e., nucleic acids). Typically a plasmid contains an origin of replication which is functional in bacterial host cells, e.g., Escherichia coli, and selectable markers for detecting bacterial host cells comprising the plasmid. Plasmids of the present invention may include genetic elements as described herein arranged such that an inserted coding sequence can be transcribed and translated in eukaryotic cells. Also, the plasmid may include a sequence from a viral nucleic acid. However, such viral sequences normally are not sufficient to direct or allow the incorporation of the plasmid into a viral particle, and the plasmid is therefore a non-viral vector. In certain embodiments described herein, a plasmid is a closed circular DNA molecule.
The term “expression” refers to the biological production of a product encoded by a coding sequence. In most cases a DNA sequence, including the coding sequence, is transcribed to form a messenger-RNA (mRNA). The messenger-RNA is then translated to form a polypeptide product which has a relevant biological activity. Also, the process of expression may involve further processing steps to the RNA product of transcription, such as splicing to remove introns, and/or post-translational processing of a polypeptide product.
As used herein, the term “polypeptide” is intended to encompass a singular “polypeptide” as well as plural “polypeptides,” and comprises any chain or chains of two or more amino acids. Thus, as used herein, terms including, but not limited to “peptide,” “dipeptide,” “tripeptide,” “protein,” “amino acid chain,” or any other term used to refer to a chain or chains of two or more amino acids, are included in the definition of a “polypeptide,” and the term “polypeptide” can be used instead of, or interchangeably with any of these terms. The term further includes polypeptides which have undergone post-translational modifications, for example, glycosylation, acetylation, phosphorylation, amidation, derivatization by known protecting/blocking groups, proteolytic cleavage, or modification by non-naturally occurring amino acids.
Also included as polypeptides of the present invention are fragments, derivatives, analogs, or variants of the foregoing polypeptides, and any combination thereof. Polypeptides, and fragments, derivatives, analogs, or variants thereof of the present invention can be antigenic and immunogenic polypeptides related to influenza virus polypeptides, which are used to prevent or treat, i.e., cure, ameliorate, lessen the severity of, or prevent or reduce contagion of infectious disease caused by the influenza virus.
As used herein, an “antigenic polypeptide” or an “immunogenic polypeptide” is a polypeptide which, when introduced into a vertebrate, reacts with the vertebrate's immune system molecules, i.e., is antigenic, and/or induces an immune response in the vertebrate, i.e., is immunogenic. It is quite likely that an immunogenic polypeptide will also be antigenic, but an antigenic polypeptide, because of its size or conformation, may not necessarily be immunogenic. Examples of antigenic and immunogenic polypeptides of the present invention include, but are not limited to, e.g., HA or fragments or variants thereof, e.g., NP or fragments thereof, e.g., PB1 or fragments or variants thereof, e.g., PB2 or fragments or variants thereof, e.g., NS1 or fragments or variants thereof, e.g., NS2 or fragments or variants thereof, e.g., M1 or fragments or variants thereof, e.g., NA or fragments or variants thereof, e.g., PA or fragments or variants thereof, and e.g. M2 or fragments or variants thereof including the extracellular fragment of M2 (M2e), or e.g., any of the foregoing polypeptides or fragments fused to a heterologous polypeptide, for example, a hepatitis B core antigen. Isolated antigenic and immunogenic polypeptides of the present invention in addition to those encoded by polynucleotides of the invention, may be provided as a recombinant protein, a purified subunit, a viral vector expressing the protein, or may be provided in the form of an inactivated influenza virus vaccine, e.g., a live-attenuated virus vaccine, a heat-killed virus vaccine, etc.
An affinity threshold associated with immunogenicity in the context of HLA class II DR molecules has been delineated (see, e.g., Southwood et al. J. Immunology 160:3363-3373, 1998, and U.S. Ser. No. 60/087,192 filed May 29, 1998). In order to define a biologically significant threshold of DR binding affinity, a database of the binding affinities of 32 DR-restricted epitopes for their restricting element (i.e., the HLA molecule that binds the motif) was compiled. In approximately half of the cases (15 of 32 epitopes), DR restriction was associated with high binding affinities, i.e. binding affinity values of 100 nM or less. In the other half of the cases (16 of 32), DR restriction was associated with intermediate affinity (binding affinity values in the 100-1000 nM range). In only one of 32 cases was DR restriction associated with an IC50 of 1000 nM or greater. Thus, 1000 nM can be defined as an affinity threshold associated with immunogenicity in the context of DR molecules.
By an “isolated” influenza virus polypeptide or a fragment, variant, or derivative thereof is intended an influenza virus polypeptide or protein that is not in its natural form. No particular level of purification is required. For example, an isolated influenza virus polypeptide can be removed from its native or natural environment. Recombinantly produced influenza virus polypeptides and proteins expressed in host cells are considered isolated for purposed of the invention, as are native or recombinant influenza virus polypeptides which have been separated, fractionated, or partially or substantially purified by any suitable technique, including the separation of influenza virus virions from eggs or culture cells in which they have been propagated. In addition, an isolated influenza virus polypeptide or protein can be provided as a live or inactivated viral vector expressing an isolated influenza virus polypeptide and can include those found in inactivated influenza virus vaccine compositions. Thus, isolated influenza virus polypeptides and proteins can be provided as, for example, recombinant influenza virus polypeptides, a purified subunit of influenza virus, a viral vector expressing an isolated influenza virus polypeptide, or in the form of an inactivated or attenuated influenza virus vaccine.
The term “immunogenic carrier” as used herein refers to a first polypeptide or fragment, variant, or derivative thereof which enhances the immunogenicity of a second polypeptide or fragment, variant, or derivative thereof. Typically, an “immunogenic carrier” is fused to or conjugated to the desired polypeptide or fragment thereof. An example of an “immunogenic carrier” is a recombinant hepatitis B core antigen expressing, as a surface epitope, an immunogenic epitope of interest. See, e.g., European Patent No. EP 0385610 B1, which is incorporated herein by reference in its entirety.
In the present invention, antigenic epitopes preferably contain a sequence of at least 4, at least 5, at least 6, at least 7, at least 8, at least 9, at least 10, at least 15, at least 20, at least 25, or between about 8 to about 30 amino acids contained within the amino acid sequence of an influenza virus polypeptide of the invention, e.g., an NP polypeptide, an M1 polypeptide or an M2 polypeptide. Certain polypeptides comprising immunogenic or antigenic epitopes are at least 5, 10, 15, 20, 25, 30, 35, 40, 45, 50, 55, 60, 65, 70, 75, 80, 85, 90, 95, or 100 amino acid residues in length. Antigenic as well as immunogenic epitopes may be linear, i.e., be comprised of contiguous amino acids in a polypeptide, or may be three dimensional, i.e., where an epitope is comprised of non-contiguous amino acids which come together due to the secondary or tertiary structure of the polypeptide, thereby forming an epitope.
As to the selection of peptides or polypeptides bearing an antigenic epitope (e.g., that contain a region of a protein molecule to which an antibody or T cell receptor can bind), it is well known in that art that relatively short synthetic peptides that mimic part of a protein sequence are routinely capable of eliciting an antiserum that reacts with the partially mimicked protein. See, e.g., Sutcliffe, J. G., et al., Science 219:660-666 (1983), which is herein incorporated by reference.
Peptides capable of eliciting an immunogenic response are frequently represented in the primary sequence of a protein, can be characterized by a set of simple chemical rules, and are confined neither to immunodominant regions of intact proteins nor to the amino or carboxyl terminals. Peptides that are extremely hydrophobic and those of six or fewer residues generally are ineffective at inducing antibodies that bind to the mimicked protein; longer peptides, especially those containing proline residues, usually are effective. Sutcliffe et al., supra, at 661. For instance, 18 of 20 peptides designed according to these guidelines, containing 8-39 residues covering 75% of the sequence of the influenza virus hemagglutinin HA1 polypeptide chain, induced antibodies that reacted with the HA1 protein or intact virus; and 12/12 peptides from the MuLV polymerase and 18/18 from the rabies glycoprotein induced antibodies that precipitated the respective proteins.
Throughout this disclosure, “binding data” results are often expressed in terms of “IC50.” IC50 is the concentration of peptide in a binding assay at which 50% inhibition of binding of a reference peptide is observed. Given the conditions in which the assays are run (i.e., limiting HLA proteins and labeled peptide concentrations), these values approximate KD values. Assays for determining binding are described in detail, e.g., in PCT publications WO 94/20127 and WO 94/03205, the disclosure of each which is herein incorporated by reference. It should be noted that IC50 values can change, often dramatically, if the assay conditions are varied, and depending on the particular reagents used (e.g., HLA preparation, etc.). For example, excessive concentrations of HLA molecules will increase the apparent measured IC50 of a given ligand. Alternatively, binding is expressed relative to a reference peptide. Although as a particular assay becomes more, or less, sensitive, the IC50's of the peptides tested may change somewhat, the binding relative to the reference peptide will not significantly change. For example, in an assay run under conditions such that the IC50 of the reference peptide increases 10-fold, the IC50 values of the test peptides will also shift approximately 10-fold. Therefore, to avoid ambiguities, the assessment of whether a peptide is a good, intermediate, weak, or negative binder is generally based on its IC50, relative to the IC50 of a standard peptide. Binding may also be determined using other assay systems including those using: live cells (e.g., Ceppellini et al., Nature 339:392, 1989; Christnick et al., Nature 352:67, 1991; Busch et al., Int. Immunol. 2:443, 19990; Hill et al., J. Immunol. 147:189, 1991; del Guercio et al., J. Immunol. 154:685, 1995), cell free systems using detergent lysates (e.g., Cerundolo et al., J. Immunol. 21:2069, 1991), immobilized purified MHC (e.g., Hill et al., J. Immunol. 152, 2890, 1994; Marshall et al., J. Immunol. 152:4946, 1994), ELISA systems (e.g., Reay et al., EMBO J. 11:2829, 1992), surface plasmon resonance (e.g., Khilko et al., J. Biol. Chem. 268:15425, 1993); high flux soluble phase assays (Hammer et al., J. Exp. Med. 180:2353, 1994), and measurement of class I MHC stabilization or assembly (e.g., Ljunggren et al., Nature 346:476, 1990; Schumacher et al., Cell 62:563, 1990; Townsend et al., Cell 62:285, 1990; Parker et al., J. Immunol. 149:1896, 1992).
The designation of a residue position in an epitope as the “carboxyl terminus” or the “carboxyl terminal position” refers to the residue position at the end of the epitope that is nearest to the carboxyl terminus of a peptide, which is designated using conventional nomenclature as defined below. “C+1” refers to the residue or position immediately following the C-terminal residue of the epitope, i.e., refers to the residue flanking the C-terminus of the epitope. The “carboxyl terminal position” of the epitope occurring at the carboxyl end of the multi-epitope construct may or may not actually correspond to the carboxyl terminal end of polypeptide. In preferred embodiments, the epitopes employed in the optimized multi-epitope constructs are motif-bearing epitopes and the carboxyl terminus of the epitope is defined with respect to primary anchor residues corresponding to a particular motif.
The designation of a residue position in an epitope as “amino terminus” or “amino-terminal position” refers to the residue position at the end of the epitope which is nearest to the amino terminus of a peptide, which is designated using conventional nomenclature as defined below. “N−1” refers to the residue or position immediately adjacent to the epitope at the amino terminal end (position number 1) of an epitope. The “amino terminal position” of the epitope occurring at the amino terminal end of the multi-epitope construct may or may not actually corresponds to the amino terminal end of the polypeptide. In preferred embodiments, the epitopes employed in the optimized multi-epitope constructs are motif-bearing epitopes and the amino terminus of the epitope is defined with respect to primary anchor residues corresponding to a particular motif.
A “construct” as used herein generally denotes a composition that does not occur in nature. A construct can be produced by synthetic technologies, e.g., recombinant DNA preparation and expression or chemical synthetic techniques for nucleic or amino acids. A construct can also be produced by the addition or affiliation of one material with another such that the result is not found in nature in that form. A “multi-epitope construct” can be used interchangeably with the term “minigene” or “multi-epitope nucleic acid vaccine,” and comprises multiple epitope nucleic acids that encode peptide epitopes of any length that can bind to a molecule functioning in the immune system, preferably a class I HLA and a T-cell receptor or a class II HLA and a T-cell receptor. All of the epitope nucleic acids in a multi-epitope construct can encode class I HLA epitopes or class II HLA epitopes. Class I HLA-encoding epitope nucleic acids are referred to as CTL epitope nucleic acids, and class II HLA-encoding epitope nucleic acids are referred to as HTL epitope nucleic acids. Some multi-epitope constructs can have a subset of the multi-epitope nucleic acids encoding class I HLA epitopes and another subset of the multi-epitope nucleic acids encoding class II HLA epitopes. The CTL epitope nucleic acids preferably encode an epitope peptide of about eight to about thirteen amino acids in length, more preferably about eight to about eleven amino acids in length, and most preferably about nine amino acids in length. The HTL epitope nucleic acids can encode an epitope peptide of about six to about thirty, preferably seven to about twenty three, preferably about seven to about seventeen, and even more preferably about eleven to about fifteen, and most preferably about thirteen amino acids in length. The multi-epitope constructs described herein preferably include five or more, ten or more, fifteen or more, twenty or more, or twenty-five or more epitope nucleic acids. All of the epitope nucleic acids in a multi-epitope construct may be from one organism (e.g., the nucleotide sequence of every epitope nucleic acid may be present in HIV strains), or the multi-epitope construct may include epitope nucleic acids present in two or more different organisms (e.g., some epitopes from HIV and some from HCV). As described hereafter, one or more epitope nucleic acids in the multi-epitope construct may be flanked by a spacer nucleic acid.
A “multi-epitope vaccine,” which is synonymous with a “polyepitopic vaccine,” or a “multi-epitope construct” or “minigene” is a vaccine comprising multiple epitopes.
“Cross-reactive binding” indicates that a peptide is bound by more than one HLA molecule; a synonym is “degenerate binding.”
A “cryptic epitope” elicits a response by immunization with an isolated peptide, but the response is not cross-reactive in vitro when intact whole protein that comprises the epitope is used as an antigen.
A “dominant epitope” is an epitope that induces an immune response upon immunization with a whole native antigen (see, e.g., Sercarz, et al., Annu. Rev. Immunol. 11:729-766, 1993). Such a response is cross-reactive in vitro with an isolated peptide epitope.
A “subdominant epitope” is an epitope which evokes little or no response upon immunization with whole antigens which comprise the epitope, but for which a response can be obtained by immunization with an isolated epitope, and this response (unlike the case of cryptic epitopes) is detected when whole protein is used to recall the response in vitro or in vivo.
With regard to a particular amino acid sequence, an “epitope” is a set of amino acid residues which is involved in recognition by a particular immunoglobulin, or in the context of T cells, those residues necessary for recognition by T cell receptor proteins and/or Major Histocompatibility Complex (MHC) receptors. In an immune system setting, in vitro or in vivo, an epitope is the collective features of a molecule, such as primary, secondary and tertiary peptide structure, and charge, that together form a site recognized by an immunoglobulin, T cell receptor or HLA molecule. Throughout this disclosure epitope and peptide are often used interchangeably. It is to be appreciated, however, that isolated or purified protein or peptide molecules larger than and comprising an epitope of the invention are still within the bounds of the invention.
A “flanking residue” is a residue that is positioned next to an epitope. A flanking residue can be introduced or inserted at a position adjacent to the N-terminus or the C-terminus of an epitope.
An “immunogenic peptide” or “peptide epitope” or “epitope” is a peptide that comprises an allele-specific motif or supermotif such that the peptide will bind an HLA molecule and induce a CTL and/or HTL response. Thus, immunogenic peptides of the invention are capable of binding to an appropriate HLA molecule and thereafter inducing a cytotoxic T cell response, or a helper T cell response, to the antigen from which the immunogenic peptide is derived.
“Heteroclitic analogs” are defined herein as a peptide with increased potency for a specific T cell, as measured by increased responses to a given dose, or by a requirement of lesser amounts to achieve the same response. Advantages of heteroclitic analogs include that the epitopes can be more potent, or more economical (since a lower amount is required to achieve the same effect). In addition, modified epitopes might overcome antigen-specific T cell unresponsiveness (T cell tolerance).
“Human Leukocyte Antigen” or “HLA” is a human class I or class II Major Histocompatibility Complex (MHC) protein (see, e.g., Stites, et al., Immunology, 8th ed., Lange Publishing, Los Altos, Calif. (1994)).
An “HLA supertype or HLA family,” as used herein, describes sets of HLA molecules grouped based on shared peptide-binding specificities. HLA class I molecules that share similar binding affinity for peptides bearing certain amino acid motifs are grouped into such HLA supertypes. The terms HLA superfamily, HLA supertype family, HLA family, and HLA xx-like molecules (where xx denotes a particular HLA type), are synonyms. HLA types, include, for example, HLA-A1, -A2, A3/A11, -A24, -B7, B44.
As used herein, “high affinity” with respect to HLA class I molecules is defined as binding with an IC50, or KD value, of 50 nM or less; “intermediate affinity” with respect to HLA class I molecules is defined as binding with an IC50 or KD value of between about 50 and about 500 nM. “High affinity” with respect to binding to HLA class II molecules is defined as binding with an IC50 or KD value of 100 nM or less; “intermediate affinity” with respect to binding to HLA class II molecules is defined as binding with an IC50 or KD value of between about 100 and about 1000 nM.
An “IC50” is the concentration of peptide in a binding assay at which 50% inhibition of binding of a reference peptide is observed. Depending on the conditions in which the assays are run (i.e., limiting HLA proteins and labeled peptide concentrations), these values may approximate KD values.
The terms “identical” or percent “identity,” in the context of two or more peptide sequences, refer to two or more sequences or subsequences that are the same or have a specified percentage of amino acid residues that are the same, when compared and aligned for maximum correspondence over a comparison window, as measured using a sequence comparison algorithm or by manual alignment and visual inspection.
“Introducing” an amino acid residue at a particular position in a multi-epitope construct, e.g., adjacent, at the C-terminal side, to the C-terminus of the epitope, encompasses configuring multiple epitopes such that a desired residue is at a particular position, e.g., adjacent to the epitope, or such that a deleterious residue is not adjacent to the C-terminus of the epitope. The term also includes inserting an amino acid residue, preferably a preferred or intermediate amino acid residue, at a particular position. An amino acid residue can also be introduced into a sequence by substituting one amino acid residue for another. Preferably, such a substitution is made in accordance with analoging principles set forth, e.g., in PCT application number PCT/US00/19774.
The phrases “isolated” or “biologically pure” refer to material that is substantially or essentially free from components which normally accompany the material as it is found in its native state. Thus, isolated peptides in accordance with the invention preferably do not contain materials normally associated with the peptides in their in situ environment.
“Link” or “join” refers to any method known in the art for functionally connecting peptides, including, without limitation, recombinant fusion, covalent bonding, disulfide bonding, ionic bonding, hydrogen bonding, and electrostatic bonding.
“Major Histocompatibility Complex” or “MHC” is a cluster of genes that plays a role in control of the cellular interactions responsible for physiologic immune responses. In humans, the MHC complex is also known as the HLA complex. For a detailed description of the MHC and HLA complexes, see, Paul, Fundamental Immunology, 3rd ed., Raven Press, New York, 1993.
As used herein, “middle of the peptide” is a position in a peptide that is neither an amino nor a carboxyl terminus.
A “minimal number of junctional epitopes” as used herein refers to a number of junctional epitopes that is lower than what would be created using a random selection criteria.
The term “motif” refers to the pattern of residues in a peptide of defined length, usually a peptide of from about 8 to about 13 amino acids for a class I HLA motif and from about 6 to about 25 amino acids for a class II HLA motif, which is recognized by a particular HLA molecule. Peptide motifs are typically different for each protein encoded by each human HLA allele and differ in the pattern of the primary and secondary anchor residues.
A “supermotif” is an amino acid sequence for a peptide that provides binding specificity shared by HLA molecules encoded by two or more HLA alleles. Preferably, a supermotif-bearing peptide is recognized with high or intermediate affinity (as defined herein) by two or more HLA antigens.
The term “peptide” is used interchangeably with “oligopeptide” in the present specification to designate a series of residues, typically L-amino acids, connected one to the other, typically by peptide bonds between the α-amino and carboxyl groups of adjacent amino acids. The preferred CTL-inducing peptides of the invention are 13 residues or less in length and usually consist of between about 8 and about 11 residues, preferably 9 or 10 residues. The preferred HTL-inducing peptides are less than about 50 residues in length and usually consist of between about 6 and about 30 residues, more usually between about 12 and 25, and often between about 15 and 20 residues.
The term “HTL epitope” refers to a peptide of defined length that can be from about 6 to about 30 amino acids in length, from about 8 to about 30 amino acids in length, from about 10 to about 30 amino acids, from about 12 to about 30 amino acids in length, from about 6 to about 25 amino acids in length, from about 8 to about 25 amino acids in length, from about 10 to about 25 amino acids, from about 12 to about 25 amino acids in length, from about 6 to about 18 amino acids in length, from about 8 to about 18 amino acids in length, from about 10 to about 18 amino acids, or from about 12 to about 18 amino acids in length, which is recognized by a particular HLA molecule.
A “PanDR binding peptide or pan-DR binding epitope” is a member of a family of molecules that binds more than one HLA class II DR molecule. The pattern that defines this family of molecules can be thought of as an HLA Class II supermotif. For example, PADRE® binds to most HLA-DR molecules and stimulates in vitro and in vivo human helper T lymphocyte (HTL) responses.
A “negative binding residue” or “deleterious residue” is an amino acid which, if present at certain positions (typically not primary anchor positions) in a peptide epitope, results in decreased binding affinity of the peptide for the peptide's corresponding HLA molecule.
“Optimizing” refers to increasing the immunogenicity or antigenicity of a multi-epitope construct having at least one epitope pair by sorting epitopes to minimize the occurrence of junctional epitopes, inserting flanking residues that flank the C-terminus or N-terminus of an epitope, and inserting spacer residue to further prevent the occurrence of junctional epitopes or to provide a flanking residue. An increase in immunogenicity or antigenicity of an optimized multi-epitope construct is measured relative to a multi-epitope construct that has not been constructed based on the optimization parameters and is using assays known to those of skill in the art, e.g., assessment of immunogenicity in HLA transgenic mice, ELISPOT, inteferon-gamma release assays, tetramer staining, chromium release assays, and presentation on dendritic cells.
“Pathogenic virus strain” is used herein to refer to any virus strain that is capable of causing disease; preferably, the virus is on the current World Health Organization (WHO), Centers for Disease Control and Prevention (CDC), Food and Drug Administration (FDA) or other public health authority list of likely circulating viruses; more preferably, the virus has been indicated as one of the three annual viral strains for inclusion in an influenza annual vaccine (i.e., “seasonal strains”). This information is readily available from these agencies, e.g., at http://www.fda.gov/cber/flu/flu.htm or at http://www.who.int/csr/disease/influenza/vaccinerecommendationsl/en/index.html.
“Pharmaceutically acceptable” refers to a generally non-toxic, inert, and/or physiologically compatible composition.
“Presented to an HLA Class I processing pathway” means that the multi-epitope constructs are introduced into a cell such that they are largely processed by an HLA Class I processing pathway. Typically, multi-epitope constructs are introduced into the cells using expression vectors that encode the multi-epitope constructs. HLA Class II epitopes that are encoded by such a multi-epitope construct are also presented on Class II molecules, although the mechanism of entry of the epitopes into the Class II processing pathway is not defined.
A “primary anchor residue” or a “primary MHC anchor” is an amino acid at a specific position along a peptide sequence that is understood to provide a contact point between the immunogenic peptide and the HLA molecule. One to three, usually two, primary anchor residues within a peptide of defined length generally defines a “motif” for an immunogenic peptide. These residues are understood to fit in close contact with peptide binding grooves of an HLA molecule, with their side chains buried in specific pockets of the binding grooves themselves. In one embodiment, for example, the primary anchor residues of an HLA class I epitope are located at position 2 (from the amino terminal position) and at the carboxyl terminal position of a 9-residue peptide epitope in accordance with the invention. The primary anchor positions for each motif and supermotif are described, for example, in Tables I and III of PCT/US00/27766, or PCT/US00/19774, the disclosure of each which is herein incorporated by reference. Preferred amino acids that can serve as in the anchors for most Class II epitopes consist of M and F in position one and V, M, S, T, A and C in position six. Tolerated amino acids that can occupy these positions for most Class II epitopes consist of L, I, V, W, and Y in position one and P, L and I in position six. The presence of these amino acids in positions one and six in Class II epitopes defines the HLA-DR1, 4, 7 supermotif. The HLA-DR3 binding motif is defined by preferred amino acids from the group of L, I, V, M, F, Y and A in position one and D, E, N, Q, S and T in position four and K, R and H in position six. Other amino acids may be tolerated in these positions but they are not preferred.
Furthermore, analog peptides can be created by altering the presence or absence of particular residues in these primary anchor positions. Such analogs are used to modulate the binding affinity of a peptide comprising a particular motif or supermotif
“Promiscuous recognition” occurs where a distinct peptide is recognized by the same T cell clone in the context of various HLA molecules. Promiscuous recognition or binding is synonymous with cross-reactive binding.
A “protective immune response” or “therapeutic immune response” refers to a CTL and/or an HTL response to an antigen derived from an infectious agent or a tumor antigen, which in some way prevents or at least partially arrests disease symptoms, side effects or progression. The immune response may also include an antibody response that has been facilitated by the stimulation of helper T cells.
The term “residue” refers to an amino acid or amino acid mimetic incorporated into a peptide or protein by an amide bond or amide bond mimetic.
A “secondary anchor residue” is an amino acid at a position other than a primary anchor position in a peptide that may influence peptide binding. A secondary anchor residue occurs at a significantly higher frequency amongst bound peptides than would be expected by random distribution of amino acids at one position. The secondary anchor residues are said to occur at “secondary anchor positions.” A secondary anchor residue can be identified as a residue which is present at a higher frequency among high or intermediate affinity binding peptides, or a residue otherwise associated with high or intermediate affinity binding. For example, analog peptides can be created by altering the presence or absence of particular residues in these secondary anchor positions. Such analogs are used to finely modulate the binding affinity of a peptide comprising a particular motif or supermotif. The terminology “fixed peptide” is sometimes used to refer to an analog peptide.
“Sorting epitopes” refers to determining or designing an order of the epitopes in a multi-epitope construct.
A “spacer” refers to a sequence that is inserted between two epitopes in a multi-epitope construct to prevent the occurrence of junctional epitopes and/or to increase the efficiency of processing. A multi-epitope construct may have one or more spacer nucleic acids. A spacer nucleic acid may flank each epitope nucleic acid in a construct, or the spacer nucleic acid to epitope nucleic acid ratio may be about 2 to 10, about 5 to 10, about 6 to 10, about 7 to 10, about 8 to 10, or about 9 to 10, where a ratio of about 8 to 10 has been determined to yield favorable results for some constructs.
The spacer nucleic acid may encode one or more amino acids. A spacer nucleic acid flanking a class I HLA epitope in a multi-epitope construct is preferably between one and about eight amino acids in length. A spacer nucleic acid flanking a class II HLA epitope in a multi-epitope construct is preferably greater than five, six, seven, or more amino acids in length, and more preferably five or six amino acids in length.
The number of spacers in a construct, the number of amino acids in a spacer, and the amino acid composition of a spacer can be selected to optimize epitope processing and/or minimize junctional epitopes. It is preferred that spacers are selected by concomitantly optimizing epitope processing and junctional motifs. Suitable amino acids for optimizing epitope processing are described herein. Also, suitable amino acid spacing for minimizing the number of junctional epitopes in a construct are described herein for class I and class II HLAs. For example, spacers flanking class II HLA epitopes preferably include G, P, and/or N residues as these are not generally known to be primary anchor residues (see, e.g., PCT/US00/19774). A particularly preferred spacer for flanking a class II HLA epitope includes alternating G and P residues, for example, (GP)n, (PG)n, (GP)nG, (PG)nP, and so forth, where n is an integer between one and ten, preferably two or about two, and where a specific example of such a spacer is GPGPG or PGPGP. A preferred spacer, particularly for class I HLA epitopes, comprises one, two, three or more consecutive alanine (A) residues.
In some multi-epitope constructs, it is sufficient that each spacer nucleic acid encodes the same amino acid sequence. In multi-epitope constructs having two spacer nucleic acids encoding the same amino acid sequence, the spacer nucleic acids encoding those spacers may have the same or different nucleotide sequences, where different nucleotide sequences may be preferred to decrease the likelihood of unintended recombination events when the multi-epitope construct is inserted into cells.
In other multi-epitope constructs, one or more of the spacer nucleic acids may encode different amino acid sequences. While many of the spacer nucleic acids may encode the same amino acid sequence in a multi-epitope construct, one, two, three, four, five or more spacer nucleic acids may encode different amino acid sequences, and it is possible that all of the spacer nucleic acids in a multi-epitope construct encode different amino acid sequences. Spacer nucleic acids may be optimized with respect to the epitope nucleic acids they flank by determining whether a spacer sequence will maximize epitope processing and/or minimize junctional epitopes, as described herein.
Multi-epitope constructs may be distinguished from one another according to whether the spacers in one construct optimize epitope processing or minimize junctional epitopes over another construct, and preferably, constructs may be distinguished where one construct is concomitantly optimized for epitope processing and junctional epitopes over the other. Computer assisted methods and in vitro and in vivo laboratory methods for determining whether a construct is optimized for epitope processing and junctional motifs are described herein.
“Synthetic peptide” refers to a peptide that is not naturally occurring, but is manmade using such methods as chemical synthesis or recombinant DNA technology.
A “TCR contact residue” or “T cell receptor contact residue” is an amino acid residue in an epitope that is understood to be bound by a T cell receptor; these are defined herein as not being any primary MHC anchor. T cell receptor contact residues are defined as the position/positions in the peptide where all analogs tested induce T-cell recognition relative to that induced with a wild type peptide.
The term “homology,” as used herein, refers to a degree of complementarity between two nucleotide sequences. The word “identity” may substitute for the word “homology” when a nucleic acid has the same nucleotide sequence as another nucleic acid. Sequence homology and sequence identity can also be determined by hybridization studies under high stringency and/or low stringency, and disclosed herein are nucleic acids that hybridize to the multi-epitope constructs under low stringency or under high stringency. Also, sequence homology and sequence identity can be determined by analyzing sequences using algorithms and computer programs known in the art. Such methods may be used to assess whether a nucleic acid is identical or homologous to the multi-epitope constructs disclosed herein. The invention pertains in part to nucleotide sequences having 80% or more, 85% or more, 90% or more, 95% or more, 97% or more, 98% or more, or 99% or more identity to the nucleotide sequence of a multi-epitope construct disclosed herein.
As used herein, the term “stringent conditions” refers to conditions which permit hybridization between nucleotide sequences and the nucleotide sequences of the disclosed multi-epitope constructs. Suitable stringent conditions can be defined by, for example, the concentrations of salt or formamide in the prehybridization and hybridization solutions, or by the hybridization temperature, and are well known in the art. In particular, stringency can be increased by reducing the concentration of salt, increasing the concentration of formamide, or raising the hybridization temperature. For example, hybridization under high stringency conditions could occur in about 50% formamide at about 37° C. to 42° C. In particular, hybridization could occur under high stringency conditions at 42° C. in 50% formamide, 5×SSPE, 0.3% SDS, and 200 μg/ml sheared and denatured salmon sperm DNA or at 42° C. in a solution comprising 50% formamide, 5×SSC (750 mM NaCl, 75 mM trisodium citrate), 50 mM sodium phosphate (pH 7.6), 5×Denhardt's solution, 10% dextran sulfate, and 20 μg/ml denatured, sheared salmon sperm DNA, followed by washing the filters in 0.1×SSC at about 65° C. Hybridization could occur under reduced stringency conditions in about 35% to 25% formamide at about 30° C. to 35° C. For example, reduced stringency conditions could occur at 35° C. in 35% formamide, 5×SSPE, 0.3% SDS, and 200 μg/ml sheared and denatured salmon sperm DNA. The temperature range corresponding to a particular level of stringency can be further narrowed by calculating the purine to pyrimidine ratio of the nucleic acid of interest and adjusting the temperature accordingly. Variations on the above ranges and conditions are well known in the art.
In addition to utilizing hybridization studies to assess sequence identity or sequence homology, known computer programs may be used to determine whether a particular nucleic acid is homologous to a multi-epitope construct disclosed herein. An example of such a program is the Bestfit program (Wisconsin Sequence Analysis Package, Version 8 for Unix, Genetics Computer Group, University Research Park, 575 Science Drive, Madison, Wis. 53711), and other sequence alignment programs are known in the art and may be utilized for determining whether two or more nucleotide sequences are homologous. Bestfit uses the local homology algorithm of Smith and Waterman, Advances in Applied Mathematics 2: 482-489 (1981), to find the best segment of homology between two sequences. When using Bestfit or any other sequence alignment program to determine whether a particular sequence is, for instance, 95% identical to a reference sequence, the parameters may be set such that the percentage of identity is calculated over the full length of the reference nucleotide sequence and that gaps in homology of up to 5% of the total number of nucleotides in the reference sequence are allowed.
The nomenclature used to describe peptide compounds follows the conventional practice wherein the amino group is presented to the left (the N-terminus) and the carboxyl group to the right (the C-terminus) of each amino acid residue. When amino acid residue positions are referred to in an epitope, they are numbered in an amino to carboxyl direction with position one being the position closest to the amino terminal end of the epitope, or the peptide or protein of which it may be a part. In the formulae representing selected specific embodiments of the present invention, the amino- and carboxyl-terminal groups, although not specifically shown, are in the form they would assume at physiologic pH values, unless otherwise specified. In the amino acid structure formulae, each residue is generally represented by standard three-letter or single-letter designations. The L-form of an amino acid residue is represented by a capital single letter or a capital first letter of a three-letter symbol, and the D-form for those amino acids having D-forms is represented by a lower case single letter or a lower case three letter symbol. Glycine has no asymmetric carbon atom and is simply referred to as “Gly” or G.
Amino acid “chemical characteristics” are defined as: Aromatic (F, W, Y); Aliphatic-hydrophobic (L, I, V, M); Small polar (S, T, C); Large polar (Q, N); Acidic (D, E); Basic (R, H, K); Proline; Alanine; and Glycine.
Acronyms used herein are as follows:
In particular embodiments to prevent HTL junctional epitopes, a spacer composed of amino acid residues that do not correspond to any known HLA Class II anchor residue, are used, e.g., alternating G and P residues (a GP spacer) is included between two HTL epitopes.
Another aspect of the invention, (consideration (ii) above) involves the introduction or substitution of particular amino acid residues at positions that flank epitopes, e.g., a position immediately adjacent to the C-terminus of the epitope, thereby generating multi-epitope constructs with enhanced antigenicity and immunogenicity compared to constructs that do not contain the particular residue introduced or substituted at that site, i.e., non-optimized multi-epitope constructs. The methods of optimizing multi-epitope constructs comprise a step of introducing a flanking residue, preferably K, N, G, R, or A at the C+1 position of the epitope, i.e., the position immediately adjacent to the C-terminus of the epitope. In an alternative embodiment, residues that contribute to decreased immunogenicity, i.e., negatively charged residues, e.g., D, aliphatic residues (I, L, M, V) or aromatic non-tryptophan residues, are replaced. The flanking residue can be introduced by positioning appropriate epitopes to provide the favorable flanking residue, or by inserting a specific residue.
Preparation of Multi-Epitope Constructs
Epitopes for inclusion in the multi-epitope constructs typically bear HLA Class I or Class II binding motifs as described, for example, in PCT applications PCT/US00/27766, or PCT/US00/19774. Multi-epitope constructs can be prepared according to the methods set forth in Ishioka, et al., J Immunol 162(7):3915-3925 (1999), for example, the disclosure of which is herein incorporated by reference.
Multiple HLA class II or class I epitopes present in a multi-epitope construct can be derived from the same antigen, or from different antigens. For example, a multi-epitope construct can contain one or more HLA epitopes that can be derived from two different antigens of the same virus or from two different antigens of different viruses. Epitopes for inclusion in a multi-epitope construct can be selected by one of skill in the art, e.g., by using a computer to select epitopes that contain HLA allele-specific motifs or supermotifs. The multi-epitope constructs of the invention also encode one or more broadly cross-reactive binding, or universal, HLA class II epitopes, i.e., pan-DR binding epitopes, e.g., PADRE®. (Epimmune, San Diego, Calif.), (described, for example, in U.S. Pat. No. 5,736,142) or a PADRE® family molecule.
Universal HLA Class II epitopes can be advantageously combined with other HLA Class I and Class II epitopes to increase the number of cells that are activated in response to a given antigen and provide broader population coverage of HLA-reactive alleles. Thus, the multi-epitope constructs of the invention can include HLA epitopes specific for an antigen, universal HLA class II epitopes, or a combination of specific HLA epitopes and at least one universal HLA class II epitope.
HLA Class I epitopes are generally about 8 to about 13 amino acids in length, in particular 8, 9, 10, or 11 amino acids in length. HLA Class II epitopes are generally about 6 to 25 amino acids in length, in particular about 13 to 21 amino acids in length. An HLA Class I or II epitope can be derived from any desired antigen of interest. The antigen of interest can be a viral antigen, surface receptor, tumor antigen, oncogene, enzyme, or any pathogen, cell or molecule for which an immune response is desired. Epitopes can be selected based on their ability to bind one or multiple HLA alleles. Epitopes that are analogs of naturally occurring sequences can also be included in the multi-epitope constructs described herein. Such analog peptides are described, for example, in PCT applications PCT/US97/03778, PCT/US00/19774, and co-pending U.S. Ser. No. 09/260,714 filed Mar. 1, 1999.
Influenza epitopes of the present invention were obtained from the H5N1 (AF036362) and H2N2 (M25924) viral protein sequences which were scanned for HLA-DR1 and -DR3 motifs using computer algorithm analysis as previously described. Approximately 1,200 sequences bearing the appropriate motifs were identified. In order to select potential epitopes that would be cross-reactive amongst a variety of influenza strains, these sequences were compared to other viral strains, typically 11 to 20, and conserved sequences were selected for peptide synthesis. Peptide binding assays were performed using peptide and purified HLA molecules. Binding analyses of 157 conserved peptides are provided in Table 3. In order to select epitopes that would be cross-reactive amongst various humans to obtain maximal population coverage, the number of vaccine candidate peptides was subsequently reduced to 53 by selecting only degenerate binding peptides demonstrating at least high to intermediate binding to greater than 60% of the purified HLA molecules tested, provided in Table 4. These 53 candidate peptides are again reduced to 1-10 HTL peptides for inclusion in the HA vaccine. The selection of these 1-10 HTL peptides is based on obtaining positive immune responses in human and mouse recall assays. A preference is also given for inclusion of peptides representing each of the 10 influenza proteins.
Multi-epitope constructs can be generated using methodology well known in the art. For example, polypeptides comprising the multi-epitope constructs can be synthesized and linked. Typically, multi-epitope constructs are constructed using recombinant DNA technology.
Expression Vectors and Construction of a Multi-Epitope Constructs
The multi-epitope constructs of the invention are typically provided as an expression vector comprising a nucleic acid encoding the multi-epitope polypeptide. Construction of such expression vectors is described, for example in PCT/US99/10646, the disclosure of which is herein incorporated by reference. The expression vectors contain at least one promoter element that is capable of expressing a transcription unit encoding the nucleic acid in the appropriate cells of an organism so that the antigen is expressed and targeted to the appropriate HLA molecule. For example, for administration to a human, a promoter element that functions in a human cell is incorporated into the expression vector.
In preferred embodiments, the invention utilizes routine techniques in the field of recombinant genetics. Basic texts disclosing the general methods of use in this invention include Sambrook et al., Molecular Cloning, A Laboratory Manual (2nd ed. 1989); Kriegler, Gene Transfer and Expression: A Laboratory Manual (1990); and Current Protocols in Molecular Biology (Ausubel et al., eds., 1994); Oligonucleotide Synthesis. A Practical Approach (Gait, ed., 1984); Kuijpers, Nucleic Acids Research 18(17):5197 (1994); Dueholm, J. Org. Chem. 59:5767-5773 (1994); Methods in Molecular Biology, volume 20 (Agrawal, ed.); and Tijssen, Laboratory Techniques in Biochemistry and Molecular Biology—Hybridization with Nucleic Acid Probes, e.g., Part I, chapter 2 “Overview of principles of hybridization and the strategy of nucleic acid probe assays” (1993)).
The nucleic acids encoding the epitopes are assembled in a construct according to standard techniques. In general, the nucleic acid sequences encoding multi-epitope polypeptides are isolated using amplification techniques with oligonucleotide primers, or are chemically synthesized. Recombinant cloning techniques can also be used when appropriate. Oligonucleotide sequences are selected which either amplify (when using PCR to assemble the construct) or encode (when using synthetic oligonucleotides to assemble the construct) the desired epitopes.
Amplification techniques using primers are typically used to amplify and isolate sequences encoding the epitopes of choice from DNA or RNA (see U.S. Pat. Nos. 4,683,195 and 4,683,202; PCR Protocols: A Guide to Methods and Applications (Innis et al., eds, 1990)). Methods such as polymerase chain reaction (PCR) and ligase chain reaction (LCR) can be used to amplify epitope nucleic acid sequences directly from mRNA, from cDNA, from genomic libraries or cDNA libraries. Restriction endonuclease sites can be incorporated into the primers. Multi-epitope constructs amplified by the PCR reaction can be purified from agarose gels and cloned into an appropriate vector.
Synthetic oligonucleotides can also be used to construct multi-epitope constructs. This method is performed using a series of overlapping oligonucleotides, representing both the sense and non-sense strands of the gene. These DNA fragments are then annealed, ligated and cloned. Oligonucleotides that are not commercially available can be chemically synthesized according to the solid phase phosphoramidite triester method first described by Beaucage & Caruthers, Tetrahedron Letts. 22:1859-1862 (1981), using an automated synthesizer, as described in Van Devanter et al., Nucleic Acids Res., 12:6159-6168 (1984). Purification of oligonucleotides is by either native acrylamide gel electrophoresis or by anion-exchange HPLC as described in Pearson & Reanier, J. Chrom. 255:137-149 (1983).
The epitopes of the multi-epitope constructs are typically subcloned into an expression vector that contains a strong promoter to direct transcription, as well as other regulatory sequences such as enhancers and polyadenylation sites. Suitable promoters are well known in the art and described, e.g., in Sambrook et al. and Ausubel et al. Eukaryotic expression systems for mammalian cells are well known in the art and are commercially available. Such promoter elements include, for example, cytomegalovirus (CMV), Rous sarcoma virus LTR and SV40.
The expression vector typically contains a transcription unit or expression cassette that contains all the additional elements required for the expression of the multi-epitope construct in host cells. A typical expression cassette thus contains a promoter operably linked to the multi-epitope construct and signals required for efficient polyadenylation of the transcript. Additional elements of the cassette may include enhancers and introns with functional splice donor and acceptor sites.
In addition to a promoter sequence, the expression cassette can also contain a transcription termination region downstream of the structural gene to provide for efficient termination. The termination region may be obtained from the same gene as the promoter sequence or may be obtained from different genes.
The particular expression vector used to transport the genetic information into the cell is not particularly critical. Any of the conventional vectors used for expression in eukaryotic cells may be used. Expression vectors containing regulatory elements from eukaryotic viruses are typically used in eukaryotic expression vectors, e.g., SV40 vectors, CMV vectors, papilloma virus vectors, and vectors derived from Epstein Bar virus.
The multi-epitope constructs of the invention can be expressed from a variety of vectors including plasmid vectors as well as viral or bacterial vectors. Examples of viral expression vectors include attenuated viral hosts, such as vaccinia or fowlpox. As an example of this approach, vaccinia virus is used as a vector to express nucleotide sequences that encode the peptides of the invention. Upon introduction into a host bearing a tumor, the recombinant vaccinia virus expresses the immunogenic peptide, and thereby elicits a host CTL and/or HTL response. Vaccinia vectors and methods useful in immunization protocols are described in, e.g., U.S. Pat. No. 4,722,848.
A wide variety of other vectors useful for therapeutic administration or immunization, e.g. adeno and adeno-associated virus vectors, retroviral vectors, non-viral vectors such as BCG (Bacille Calmette Guerin), Salmonella typhi vectors, detoxified anthrax toxin vectors, and the like, will be apparent to those skilled in the art.
Immunogenicity and antigenicity of the multi-epitope constructs are evaluated as described herein.
Targeting Sequences
The expression vectors of the invention may encode one or more MHC epitopes operably linked to a MHC targeting sequence, and are referred to herein as “targeting nucleic acids” or “targeting sequences.” The use of a MHC targeting sequence enhances the immune response to an antigen, relative to delivery of antigen alone, by directing the peptide epitope to the site of MHC molecule assembly and transport to the cell surface, thereby providing an increased number of MHC molecule-peptide epitope complexes available for binding to and activation of T cells.
MHC Class I targeting sequences can be used in the present invention, e.g., those sequences that target an MHC Class I epitope peptide to a cytosolic pathway or to the endoplasmic reticulum (see, e.g., Rammensee et al., Immunogenetics 41:178-228 (1995)). For example, the cytosolic pathway processes endogenous antigens that are expressed inside the cell. Although not wishing to be bound by any particular theory, cytosolic proteins are thought to be at least partially degraded by an endopeptidase activity of a proteosome and then transported to the endoplasmic reticulum by the TAP molecule (transporter associated with processing). In the endoplasmic reticulum, the antigen binds to MHC Class I molecules. Endoplasmic reticulum signal sequences bypass the cytosolic processing pathway and directly target endogenous antigens to the endoplasmic reticulum, where proteolytic degradation into peptide fragments occurs. Such MHC Class I targeting sequences are well known in the art, and include, e.g., signal sequences such as those from Ig kappa, tissue plasminogen activator or insulin. A preferred signal peptide is the human. Ig kappa chain sequence. Endoplasmic reticulum signal sequences can also be used to target MHC Class II epitopes to the endoplasmic reticulum, the site of MHC Class I molecule assembly. MHC Class II targeting sequences can also be used in the invention, e.g., those that target a peptide to the endocytic pathway. These targeting sequences typically direct extracellular antigens to enter the endocytic pathway, which results in the antigen being transferred to the lysosomal compartment where the antigen is proteolytically cleaved into antigen peptides for binding to MHC Class II molecules. As with the normal processing of exogenous antigen, a sequence that directs a MHC Class II epitope to the endosomes of the endocytic pathway and/or subsequently to lysosomes, where the MHC Class II epitope can bind to a MHC Class II molecule, is a MHC Class II targeting sequence. For example, group of MHC Class II targeting sequences useful in the invention are lysosomal targeting sequences, which localize polypeptides to lysosomes. Since MHC Class II molecules typically bind to antigen peptides derived from proteolytic processing of endocytosed antigens in lysosomes, a lysosomal targeting sequence can function as a MHC Class II targeting sequence. Lysosomal targeting sequences are well known in the art and include sequences found in the lysosomal proteins LAMP-1 and LAMP-2 as described by August et al. U.S. Pat. No. 5,633,234, issued May 27, 1997), which is incorporated herein by reference.
Other lysosomal proteins that contain lysosomal targeting sequences include HLA-DM. HLA-DM is an endosomal/lysosomal protein that functions in facilitating binding of antigen peptides to MHC Class II molecules. Since it is located in the lysosome, HLA-DM has a lysosomal targeting sequence that can function as a MHC Class II molecule targeting sequence (Copier et al., J. Immunol. 157:1017-1027 (1996), which is incorporated herein by reference).
The resident lysosomal protein HLA-DO can also function as a lysosomal targeting sequence. In contrast to the above described resident lysosomal proteins LAMP-1 and HLA-DM, which encode specific Tyr-containing motifs that target proteins to lysosomes, HLA-DO is targeted to lysosomes by association with HLA-DM (Liljedahl et al., EMBO J., 15:4817-4824 (1996)), which is incorporated herein by reference. Therefore, the sequences of HLA-DO that cause association with HLA-DM and, consequently, translocation of HLA-DO to lysosomes can be used as MHC Class II targeting sequences. Similarly, the murine homolog of HLA-DO, H2-DO, can be used to derive a MHC Class II targeting sequence. A MHC Class II epitope can be fused to HLA-DO or H2-DO and targeted to lysosomes.
In another example, the cytoplasmic domains of B cell receptor subunits Ig-α and Ig-β mediate antigen internalization and increase the efficiency of antigen presentation as described in, for example, Bonnerot et al., Immunity, 3:335-347 (1995). Therefore, the cytoplasmic domains of the Ig-α and Ig-β proteins can function as MHC Class II targeting sequences that target a MHC Class II epitope to the endocytic pathway for processing and binding to MHC Class II molecules.
Another example of a MHC Class II targeting sequence that directs MHC Class II epitopes to the endocytic pathway is a sequence that directs polypeptides to be secreted, where the polypeptide can enter the endosomal pathway. These MHC Class II targeting sequences that direct polypeptides to be secreted mimic the normal pathway by which exogenous, extracellular antigens are processed into peptides that bind to MHC Class II molecules. Any signal sequence that functions to direct a polypeptide through the endoplasmic reticulum and ultimately to be secreted can function as a MHC Class II targeting sequence so long as the secreted polypeptide can enter the endosomal/lysosomal pathway and be cleaved into peptides that can bind to MHC Class II molecules.
In another example, the Ii protein binds to MHC Class II molecules in the endoplasmic reticulum, where it functions to prevent peptides present in the endoplasmic reticulum from binding to the MHC Class II molecules. Therefore, fusion of a MHC Class II epitope to the Ii protein targets the MHC Class II epitope to the endoplasmic reticulum and a MHC Class II molecule. For example, the CLIP sequence of the Ii protein can be removed and replaced with a MHC Class II epitope sequence so that the MHC Class II epitope is directed to the endoplasmic reticulum, where the epitope binds to a MHC Class II molecule.
In some cases, antigens themselves can serve as MHC Class II or I targeting sequences and can be fused to a universal MHC Class II epitope to stimulate an immune response. Although cytoplasmic viral antigens are generally processed and presented as complexes with MHC Class I molecules, long-lived cytoplasmic proteins such as the influenza matrix protein can enter the MHC Class MHC Class II molecule processing pathway as described in, for example, Gueguen & Long, Proc. Natl. Acad. Sci. USA, 93:14692-14697 (1996). Therefore, long-lived cytoplasmic proteins can function as a MHC Class MHC Class II targeting sequence. For example, an expression vector encoding influenza matrix protein fused to a universal MHC Class I/MHC Class II epitope can be advantageously used to target influenza antigen and the universal MHC Class I/MHC Class II epitope to the MHC Class I/MHC Class II pathway for stimulating an immune response to influenza.
Other examples of antigens functioning as MHC Class I/MHC Class II targeting sequences include polypeptides that spontaneously form particles. The polypeptides are secreted from the cell that produces them and spontaneously form particles, which are taken up into an antigen-presenting cell by endocytosis such as receptor-mediated endocytosis or are engulfed by phagocytosis. The particles are proteolytically cleaved into antigen peptides after entering the endosomal/lysosomal pathway.
One such polypeptide that spontaneously forms particles is HBV surface antigen (HBV-S) as described in, for example, Diminsky et al., Vaccine 15:637-647 (1997) or Le Borgne et al., Virology, 240:304-315 (1998). Another polypeptide that spontaneously forms particles is HBV core antigen as described in, for example, Kuhrober et al., International Immunol., 9:1203-1212 (1997). Still another polypeptide that spontaneously forms particles is the yeast Ty protein as described in, for example, Weber et al., Vaccine, 13:831-834 (1995). For example, an expression vector containing HBV-S antigen fused to a universal MHC Class MHC Class II epitope can be advantageously used to target HBV-S antigen and the universal MHC Class MHC Class II epitope to the MHC Class MHC Class II pathway for stimulating an immune response to HBV.
The Minimization of Junctional Motifs
One of the considerations in designing multi-epitope constructs is the inadvertent creation of junctional epitopes when placing epitopes adjacent to each other. The presence of such epitopes in a multi-epitope construct could significantly affect performance. Strategies to guard against this undesired effect are disclosed herein for application to the development of multi-epitope vaccines. Junctional epitopes can first be minimized by sorting the epitopes to identify an order in which the numbers of junctional epitopes is minimized. Such a sorting procedure can be performed using a computer or by eye, if necessary, or depending on the number of epitopes to be included in the multi-epitope construct.
Eliminating Class II Junctional Epitopes and Testing for Class II Restricted Responses In Vivo
As a further element in eliminating junctional epitopes, spacer sequences can be inserted between two epitopes that create a junctional epitope when juxtaposed.
In one embodiment, to correct the problem of junctional epitopes for HTL epitopes, a spacer of, for example, five amino acids in length is inserted between the two epitopes. The amino acid residues incorporated into such a spacer are preferably those amino acid residues that are not known to be primary anchor residues for any of the HLA Class II binding motifs. Such residues include G, P, and N. In a preferred embodiment, a spacer with the sequence GPGPG is inserted between two epitopes. Previous work has demonstrated that the GP spacer is particularly effective in disrupting Class II binding interactions (Sette et al., J. Immunol., 143:1268-73 (1989)). All known human Class II binding motifs and the mouse IAb (the Class II expressed by HLA transgenic mice) do not tolerate either G or P at this main anchor positions, which are spaced four residues apart. This approach virtually guarantees that no Class II restricted epitopes can be formed as junctional epitopes.
Polypeptides are synthesized incorporating influenza-derived HTL epitopes. These epitopes are broadly cross-reactive HLA DR binding epitopes. These epitopes will also efficiently bind the murine IAb Class II molecule.
Responses against multiple influenza-derived Class II epitopes can be simultaneously induced, and IAb/DR crossreactivity can be utilized to investigate the immunogenicity of various constructs incorporating HTL epitope candidates. Finally, appropriate spacers can be employed to effectively disrupt Class II junctional epitopes that would otherwise interfere with effective vaccine immunogenicity.
In the case of Class I restricted responses, one case of a naturally occurring junctional epitope and the consequent inhibition of epitope specific responses has been presented by McMichael and coworkers (Tussey et al., Immunity, 3(1):65-77 (1995)). To address the problem of junctional epitopes for Class I, similar analyses can be performed. For example, a specific computer program is employed to identify potential Class I restricted junctional epitopes, by screening for selected murine motifs and for the most common human Class I HLA A and B motifs.
Spacer sequences can also similarly be employed to prevent CTL junctional epitopes. Often, very small residues such as A or G are preferred spacer residues. G also occurs relatively infrequently as a preferred primary anchor residue (see, e.g., PCT/US00/24802) of an HLA Class I binding motif. These spacers can vary in length, e.g., spacer sequences can typically be 1, 2, 3, 4, 5, 6, 7, or 8 amino acid residues in length and are sometimes longer. Smaller lengths are often preferred because of physical constraints in producing the multi-epitope construct.
Sorting and Optimization of Multi-Epitope Constructs
To develop multi-epitope constructs using the invention, the epitopes for inclusion in the multi-epitope construct are sorted and optimized using the parameters defined herein. Sorting and optimization can be performed using a computer or, for fewer numbers of epitopes, not using a computer. Methods of sorting and optimization and disclosed in WO 02/083714, the disclosure of which is herein incorporated by reference.
Multi-epitope constructs can also be optimized by determining the structure of each construct to be considered. Macromolecular structures such as polypeptide structures can be described in terms of various levels of organization. For a general discussion of this organization, see, e.g., Alberts et al., Molecular Biology of the Cell (3rd ed., 1994) and Cantor and Schimmel, Biophysical Chemistry Part I: The Conformation of Biological Macromolecules (1980). “Primary structure” refers to the amino acid sequence of a particular peptide. “Secondary structure” refers to locally ordered, three dimensional structures within a polypeptide. These structures are commonly known as domains. Domains are portions of a polypeptide that form a compact unit of the polypeptide. Typical domains are made up of sections of lesser organization such as stretches of β-sheet and α-helices. “Tertiary structure” refers to the complete three dimensional structure of a polypeptide monomer. “Quaternary structure” refers to the three dimensional structure formed by the noncovalent association of independent tertiary units.
Structural predictions such as charge distribution, hydrophobic/hydrophilic region analysis, or folding predictions can be performed using sequence analysis programs known to those of skill in the art, for example, hydrophobic and hydrophilic domains can be identified (see, e.g., Kyte & Doolittle, J. Mol. Biol. 157:105-132 (1982) and Stryer, Biochemistry (3rd ed. 1988); see also any of a number of Internet based sequence analysis programs, such as those found at dot.imgen.bcm.tmc.edu.
A three-dimensional structural model of a multi-epitope construct can also be generated. This is generally performed by entering amino acid sequence to be analyzed into the computer system. The amino acid sequence represents the primary sequence or subsequence of the protein, which encodes the structural information of the protein. The three-dimensional structural model of the protein is then generated by the interaction of the computer system, using software known to those of skill in the art.
The amino acid sequence represents a primary structure that encodes the information necessary to form the secondary, tertiary and quaternary structure of the protein of interest. The software looks at certain parameters encoded by the primary sequence to generate the structural model. These parameters are referred to as “energy terms,” and primarily include electrostatic potentials, hydrophobic potentials, solvent accessible surfaces, and hydrogen bonding. Secondary energy terms include van der Waals potentials. Biological molecules form the structures that minimize the energy terms in a cumulative fashion. The computer program is therefore using these terms encoded by the primary structure or amino acid sequence to create the secondary structural model. The tertiary structure of the protein encoded by the secondary structure is then formed on the basis of the energy terms of the secondary structure. The user can enter additional variables such as whether the protein is membrane bound or soluble, its location in the body, and its cellular location, e.g., cytoplasmic, surface, or nuclear. These variables along with the energy terms of the secondary structure are used to form the model of the tertiary structure. In modeling the tertiary structure, the computer program matches hydrophobic faces of secondary structure with like, and hydrophilic faces of secondary structure with like. Those multi-epitope constructs that are most readily accessible to the HLA processing apparatus are then selected.
Assessment of Immunogenicity of Multi-Epitope Vaccines
The development of multi-epitope constructs represents a unique challenge, because the species-specificity of the peptide binding to MHC. Different MHC types from different species tend to bind different sets of peptides (Rammensee et al., Immunogenetics, 41(4):178-228 (1995)). As a result, it is not possible to test in regular laboratory animals a construct composed of human epitopes. Alternatives to overcome this limitation are generally available. They include: 1) testing analogous constructs incorporating epitopes restricted by non-human MHC; 2) reliance on control epitopes restricted by non human MHC; 3) reliance on crossreactivity between human and non-human MHC; 4) the use of HLA transgenic animals; and 5) antigenicity assays utilizing human cells in vivo. The following is a brief overview of the development of the technology for analyzing antigenicity and immunogenicity.
Measuring HTL Responses
In preferred embodiments, vaccine constructs are optimized to induce Class II restricted immune responses. One method of evaluating multi-epitope constructs including Class II epitopes, is to use HLA-DR transgenic mice. Several groups have produced and characterized HLA-DR transgenic mice (Taneja V., David C. S., Immunol Rev, 169:67-79 (1999)).
An alternative also exists which relies on crossreactivity between certain human MHC molecules and particular MHC molecules expressed by laboratory animals. Bertoni and colleagues (Bertoni et al., J Immunol, 161(8):4447-55 (1998)) have noted that appreciable crossreactivity can be demonstrated between certain HLA Class I supertypes and certain PATR molecules expressed by chimpanzees. Crossreactivity between human and macaques at the level of Class II (Geluk et al., J Exp Med, 177(4):979-87 (1993)) and Class I molecules (Dzuris, et al., J. Immunol., July 1999) has also been noted. Finally, it can also be noted that the motif recognized by human HLA B7 supertype is essentially the same as the one recognized by the murine Class I Ld (Rammensee et al., Immunogenetics, 41(4):178-228 (1995)). Of relevance to testing HLA DR restricted epitopes in mice, it has been shown by Wall et al. (Wall et al., J. Immunol., 152:4526-36 (1994)) that similarities exist in the motif of DR1 and IAb. We routinely breed our transgenic mice to take advantage of this fortuitous similarity. Furthermore, we have also shown that most of our peptides bind to IAb, so that we use these mice for the study of CTL and HTL immunogenicity.
Measuring and Quantitating Immune Responses from Clinical Samples
A crucial element to assess vaccine performance is to evaluate its capacity to induce immune responses in vivo. Analyses of CTL and HTL responses against the immunogen, as well as against common recall antigens are commonly used and are known in the art. Assays employed included chromium release, lymphokine secretion and lymphoproliferation assays.
More sensitive techniques such as the ELISPOT assay, intracellular cytoline staining, and tetramer staining have become available in the art. It is estimated that these newer methods are 10- to 100-fold more sensitive than the common CTL and HTL assays (Murali-Krishna et al., Immunity, 8(2): 177-87 (1998)), because the traditional methods measure only the subset of T cells that can proliferate in vitro, and may, in fact, be representative of only a fraction of the memory T cell compartment (Ogg G. S., McMichael A. J., Curr Opin Immunol, 10(4):393-6 (1998)). Specifically in the case of HIV, these techniques have been used to measure antigen-specific CTL responses from patients that would have been undetectable with previous techniques (Ogg et al., Science, 279(5359):2103-6 (1998); Gray et al., J Immunol, 162(3):1780-8 (1999); Ogg et al., J Virol, 73(11):9153-60 (1999); Kalams et al., J Viro; 73(8):6721-8 (1999); Larsson et al., AIDS, 13(7):767-77 (1999); Come et al., J Acquir Immune Defic Syndr Hum Retrovirol, 20(5):442-7 (1999)).
With relatively few exceptions, direct activity of freshly isolated cells has been difficult to demonstrate by the means of traditional assays (Ogg G. S., McMichael A. J., Curr Opin Immunol, 10(4):393-6 (1998)). However, the increased sensitivity of the newer techniques has allowed investigators to detect responses from cells freshly isolated from infected humans or experimental animals (Murali-Krishna et al., Immunity, 8(2):177-87 (1998); Ogg G. S., McMichael A. J., Curr Opin Immunol, 10(4):393-6 (1998)). The availability of these sensitive assays, that do not depend on an in vitro restimulation step, has greatly facilitated the study of CTL function in natural infection and cancer. In contrast, assays utilized as an endpoint to judge effectiveness of experimental vaccines are usually performed in conjunction with one or more in vitro restimulation steps (Ogg G. S., McMichael A. J., Curr Opin Immunol, 10(4):393-6 (1998)). In fact, with few exceptions (Hanke et al., Vaccine, 16(4):426-35 (1998)), freshly isolated Class I-restricted CD8+ T cells have been difficult to demonstrate in response to immunization with experimental vaccines designed to elicit CTL responses. The use of sensitive assays, such as ELISPOT or in situ IFNγ ELISA, have been combined with a restimulation step to achieve maximum sensitivity; MHC tetramers are also used for this purpose.
MHC tetramers were first described in 1996 by Altman and colleagues. They produced soluble HLA-A2 Class I molecules which were folded with HIV-specific peptides containing a CTL epitope complexed together into tetramers tagged with fluorescent markers. These are used to label populations of T cells from HIV-infected individuals that recognize the epitope (Ogg G. S., McMichael A. J., Curr Opin Immunol, 10(4):393-6 (1998)). These cells were then quantified by flow cytometry, providing a frequency measurement for the T cells that are specific for the epitope. This technique has become very popular in HIV research as well as in other infectious diseases (Ogg G. S., McMichael A. J., Curr Opin Immunol, 10(4):393-6 (1998); Ogg et al., Science, 279(5359):2103-6 (1998); Gray et al., J Immunol, 162(3):1780-8 (1999); Ogg et al., J Virol, 73(11):9153-60 (1999); Kalams et al., J Virol, 73(8):6721-8 (1999)). However, HLA polymorphism can limit the general applicability of this technique, in that the tetramer technology relies on defined HLA/peptide combinations. However, it has been shown that a variety of peptides, including HIV-derived peptides, are recognized by peptide-specific CTL lines in the context of different members of the A2, A3 and B7 supertypes (Threlkeld et al., J Immunol, 159(4):1648-57 (1997); Bertoni et al., J Clin Invest, 100(3):503-13 (1997)). Taken together these observations demonstrate that a T cell receptor (TCR) for a given MHC/peptide combination can have detectable affinity for the same peptide presented by a different MHC molecule from the same supertype.
In circumstances in which efficacy of a prophylactic vaccine is primarily correlated with the induction of a long-lasting memory response, restimulation assays can be the most appropriate and sensitive measures to monitor vaccine-induced immunological responses. Conversely, in the case of therapeutic vaccines, the main immunological correlate of activity can be the induction of effector T cell function, most aptly measured by primary assays. Thus, the use of sensitive assays allows for the most appropriate testing strategy for immunological monitoring of vaccine efficacy.
Antigenicity of Multi-Epitope Constructs in Transfected Human APC's
Antigenicity assays are performed to evaluate epitope processing and presentation in human cells. An episomal vector to efficiently transfect human target cells with multi-epitope nucleic acid vaccines is used to perform such an analysis.
For example, 221 A2Kb target cells were transfected with an influenza multi-epitope vaccine. The 221 A2 Kb target cell expresses the A2 Kb gene that is expressed in HLA transgenic mice, but expresses no endogenous Class I (Shimizu Y, DeMars R., J Immunol, 142(9):3320-8 (1989)). These transfected cells are assayed for their capacity to present antigen to CTL lines derived from HLA transgenic mice and specific for various HIV-derived CTL epitopes. To correct for differences in antigen sensitivity of different CTL lines, peptide dose titrations, using untransfected cells as APC, are run in parallel.
These data have several important implications. First, they suggest that different epitopes contained within a given construct may be processed and presented with differential efficiency. Second, they suggest that immunogenicity is proportional to the amount of processed epitope generated. Finally, these results provide an important validation of the use of transgenic mice for the purpose of optimization of multi-epitope vaccines destined for human use.
Methods of Administration
The invention also relates to pharmaceutical compositions comprising a pharmaceutically acceptable carrier and an expression vector of the invention or a polypeptide derived therefrom. Pharmaceutically acceptable carriers are well known in the art and include aqueous or non-aqueous solutions, suspensions and emulsions, including physiologically buffered saline, alcohol/aqueous solutions or other solvents or vehicles such as glycols, glycerol, oils such as olive oil or injectable organic esters, lipids, liposomes or virosomes.
A pharmaceutically acceptable carrier can contain physiologically acceptable compounds that act, for example, to stabilize the expression vector or increase the absorption of the expression vector. Such physiologically acceptable compounds include, for example, carbohydrates, such as glucose, sucrose or dextrans, antioxidants such as ascorbic acid or glutathione, chelating agents, low molecular weight polypeptides, antimicrobial agents, inert gases or other stabilizers or excipients. Expression vectors can additionally be complexed with other components such as peptides, polypeptides and carbohydrates. Expression vectors can also be complexed to particles or beads that can be administered to an individual, for example, using a vaccine gun. One skilled in the art would know that the choice of a pharmaceutically acceptable carrier, including a physiologically acceptable compound, depends, for example, on the route of administration of the expression vector.
The invention further relates to methods of administering a pharmaceutical composition comprising an expression vector of the invention or a polypeptide derived therefrom to stimulate an immune response. The expression vectors are administered by methods well known in the art as described in, for example, Donnelly et al. (Ann. Rev. Immunol., 15:617-648 (1997)); Felgner et al. (U.S. Pat. No. 5,580,859, issued Dec. 3, 1996); Felgner (U.S. Pat. No. 5,703,055, issued Dec. 30, 1997); and Carson et al. (U.S. Pat. No. 5,679,647, issued Oct. 21, 1997). In one embodiment, the multi-epitope construct is administered as naked nucleic acid.
A pharmaceutical composition comprising an expression vector of the invention or a polypeptide derived therefrom can be administered to stimulate an immune response in a subject by various routes including, for example, orally, intravaginally, rectally, or parenterally, such as intravenously, intramuscularly, subcutaneously, intraorbitally, intracapsularly, intraperitoneally, intracistemally or by passive or facilitated absorption through the skin using, for example, a skin patch or transdermal iontophoresis, respectively. Furthermore, the composition can be administered by injection, intubation or topically, the latter of which can be passive, for example, by direct application of an ointment or powder, or active, for example, using a nasal spray or inhalant. An expression vector also can be administered as a topical spray, in which case one component of the composition is an appropriate propellant. The pharmaceutical composition also can be incorporated, if desired, into liposomes, virosomes, microspheres or other polymer matrices as described in, for example, Felgner et al., U.S. Pat. No. 5,703,055; Gregoriadis, Liposome Technology, Vols. I to III (2nd ed. 1993). Liposomes, for example, which consist of phospholipids or other lipids, are nontoxic, physiologically acceptable and metabolizable carriers that are relatively simple to make and administer. A virosome, for example, can be an immunopotentiating reconstituted influenza virosome (IRIV).
The expression vectors of the invention or a polypeptide derived therefrom can be delivered to the interstitial spaces of tissues of an animal body as described in, for example, Felgner et al., U.S. Pat. Nos. 5,580,859 and 5,703,055. Administration of expression vectors of the invention to muscle is a particularly effective method of administration, including intradermal and subcutaneous injections and transdermal administration. Transdermal administration, such as by iontophoresis, is also an effective method to deliver expression vectors of the invention to muscle. Epidermal administration of expression vectors of the invention can also be employed. Epidermal administration involves mechanically or chemically irritating the outermost layer of epidermis to stimulate an immune response to the irritant (Carson et al., U.S. Pat. No. 5,679,647).
Other effective methods of administering an expression vector of the invention or a polypeptide derived therefrom to stimulate an immune response include mucosal administration as described in, for example, Carson et al., U.S. Pat. No. 5,679,647. For mucosal administration, the most effective method of administration includes intranasal administration of an appropriate aerosol containing the expression vector and a pharmaceutical composition. Suppositories and topical preparations are also effective for delivery of expression vectors to mucosal tissues of genital, vaginal and ocular sites. Additionally, expression vectors can be complexed to particles and administered by a vaccine gun.
The dosage to be administered is dependent on the method of administration and will generally be between about 0.1 μg up to about 200 μg. For example, the dosage can be from about 0.05 μg/kg to about 50 mg/kg, in particular about 0.005-5 mg/kg. An effective dose can be determined, for example, by measuring the immune response after administration of an expression vector. For example, the production of antibodies specific for the MHC Class II epitopes or MHC Class I epitopes encoded by the expression vector can be measured by methods well known in the art, including ELISA or other immunological assays. In addition, the activation of T helper cells or a CTL response can be measured by methods well known in the art including, for example, the uptake of 3H-thymidine to measure T cell activation and the release of 51Cr to measure CTL activity (see Examples II and III below).
The pharmaceutical compositions comprising an expression vector of the invention or a polypeptide derived therefrom can be administered to mammals, particularly humans, for prophylactic or therapeutic purposes. Diseases related to influenza virus infection can be treated or prevented using the expression vectors of the invention.
In therapeutic applications, the expression vectors of the invention or a polypeptide derived therefrom are administered to an individual already suffering from influenza virus infection or a related disease. Those in the incubation phase or acute phase of the disease can be treated with expression vectors of the invention, including those expressing all universal MHC Class II epitopes, separately or in conjunction with other treatments, as appropriate.
In therapeutic and prophylactic applications, pharmaceutical compositions comprising expression vectors of the invention or a polypeptide derived therefrom are administered to a patient in an amount sufficient to elicit an effective immune response to an antigen and to ameliorate the signs or symptoms of a disease. The amount of expression vector to administer that is sufficient to ameliorate the signs or symptoms of a disease is termed a therapeutically effective dose. The amount of expression vector sufficient to achieve a therapeutically effective dose will depend on the pharmaceutical composition comprising an expression vector of the invention, the manner of administration, the state and severity of the disease being treated, the weight and general state of health of the patient and the judgment of the prescribing physician.
The present invention also provides methods for delivering an influenza polypeptide or a fragment, variant, or derivative thereof to a human, which comprise administering to a human one or more of the compositions described herein; such that upon administration of compositions such as those described herein, an influenza polypeptide, or fragment, variant, or derivative thereof is expressed in human cells, in an amount sufficient to generate an immune response to the influenza virus or administering the influenza virus polypeptide or a fragment, variant, or derivative thereof itself to the human in an amount sufficient to generate an immune response.
The present invention further provides methods for delivering an influenza virus polypeptide or a fragment, variant, or derivative thereof to a human, which comprise administering to a vertebrate one or more of the compositions described herein; such that upon administration of compositions such as those described herein, an immune response is generated in the vertebrate.
The term “vertebrate” is intended to encompass a singular “vertebrate” as well as plural “vertebrates” and comprises mammals and birds, as well as fish, reptiles, and amphibians.
The term “mammal” is intended to encompass a singular “mammal” and plural “mammals,” and includes, but is not limited to humans; primates such as apes, monkeys (e.g., owl, squirrel, cebus, rhesus, African green, patas, cynomolgus, and cercopithecus), orangutans, baboons, gibbons, and chimpanzees; canids such as dogs and wolves; felids such as cats, lions, and tigers; equines such as horses, donkeys, and zebras, food animals such as cows, pigs, and sheep; ungulates such as deer and giraffes; ursids such as bears; and others such as rabbits, mice, ferrets, seals, whales. In particular, the mammal can be a human subject, a food animal or a companion animal.
The term “bird” is intended to encompass a singular “bird” and plural “birds,” and includes, but is not limited to feral water birds such as ducks, geese, terns, shearwaters, and gulls; as well as domestic avian species such as turkeys, chickens, quail, pheasants, geese, and ducks. The term “bird” also encompasses passerine birds such as starlings and budgerigars.
The present invention further provides a method for generating, enhancing or modulating an immune response to an influenza virus comprising administering to a vertebrate one or more of the compositions described herein. In this method, the compositions may include one or more isolated polynucleotides comprising at least one nucleic acid fragment where the nucleic acid fragment is optionally a fragment of a coding region encoding an influenza virus polypeptide, or a fragment, variant, or derivative thereof. In another embodiment, the compositions may include both a polynucleotide as described above, and also an isolated influenza virus polypeptide, or a fragment, variant, or derivative thereof, wherein the protein is provided as a recombinant protein, in particular, a fusion protein, a purified subunit, viral vector expressing the protein, or in the form of an inactivated influenza virus vaccine. Thus, the latter compositions include both a polynucleotide encoding an influenza virus polypeptide or a fragment, variant, or derivative thereof and an isolated influenza virus polypeptide or a fragment, variant, or derivative thereof. The influenza virus polypeptide or a fragment, variant, or derivative thereof encoded by the polynucleotide of the compositions need not be the same as the isolated influenza virus polypeptide or a fragment, variant, or derivative thereof of the compositions. Compositions to be used according to this method may be univalent, bivalent, trivalent or multivalent.
The polynucleotides of the compositions may comprise a fragment of a human (or other vertebrate) coding region encoding a protein of the influenza virus, or a fragment, variant, or derivative thereof. The polynucleotides are incorporated into the cells of the vertebrate in vivo, and an antigenic amount of the influenza virus polypeptide, or fragment, variant, or derivative thereof, is produced in vivo. Upon administration of the composition according to this method, the influenza virus polypeptide or a fragment, variant, or derivative thereof is expressed in the vertebrate in an amount sufficient to elicit an immune response. Such an immune response might be used, for example, to generate antibodies to the influenza virus for use in diagnostic assays or as laboratory reagents, or as therapeutic or preventative vaccines as described herein.
The present invention further provides a method for generating, enhancing, or modulating a protective and/or therapeutic immune response to influenza virus in a vertebrate, comprising administering to a vertebrate in need of therapeutic and/or preventative immunity one or more of the compositions described herein. In this method, the compositions include one or more polynucleotides comprising at least one nucleic acid fragment, where the nucleic acid fragment is optionally a fragment of a coding region encoding an influenza virus polypeptide, or a fragment, variant, or derivative thereof. In a further embodiment, the composition used in this method includes both an isolated polynucleotide comprising at least one nucleic acid fragment, where the nucleic acid fragment is optionally a fragment of a coding region encoding an influenza virus polypeptide, or a fragment, variant, or derivative thereof; and at least one isolated influenza virus polypeptide, or a fragment, variant, or derivative thereof. Thus, the latter composition includes both an isolated polynucleotide encoding an influenza virus polypeptide or a fragment, variant, or derivative thereof and an isolated influenza virus polypeptide or a fragment, variant, or derivative thereof, for example, a recombinant protein, a purified subunit, viral vector expressing the protein, or an inactivated virus vaccine. Upon administration of the composition according to this method, the influenza virus polypeptide or a fragment, variant, or derivative thereof is expressed in the human in a therapeutically or prophylactically effective amount.
As used herein, an “immune response” refers to the ability of a vertebrate to elicit an immune reaction to a composition delivered to that vertebrate. Examples of immune responses include an antibody response or a cellular, e.g., cytotoxic T-cell, response. One or more compositions of the present invention may be used to prevent influenza infection in vertebrates, e.g., as a prophylactic vaccine, to establish or enhance immunity to influenza virus in a healthy individual prior to exposure to influenza or contraction of influenza disease, thus preventing the disease or reducing the severity of disease symptoms.
As mentioned above, compositions of the present invention can be used both to prevent influenza virus infection, and also to therapeutically treat influenza virus infection. In individuals already exposed to influenza, or already suffering from influenza disease, the present invention is used to further stimulate the immune system of the vertebrate, thus reducing or eliminating the symptoms associated with that disease or disorder. As defined herein, “treatment” refers to the use of one or more compositions of the present invention to prevent, cure, retard, or reduce the severity of influenza disease symptoms in a vertebrate, and/or result in no worsening of influenza disease over a specified period of time in a vertebrate which has already been exposed to influenza virus and is thus in need of therapy. The term “prevention” refers to the use of one or more compositions of the present invention to generate immunity in a vertebrate which has not yet been exposed to a particular strain of influenza virus, thereby preventing or reducing disease symptoms if the vertebrate is later exposed to the particular strain of influenza virus. The methods of the present invention therefore may be referred to as therapeutic vaccination or preventative or prophylactic vaccination. It is not required that any composition of the present invention provide total immunity to influenza or totally cure or eliminate all influenza disease symptoms. As used herein, a “vertebrate in need of therapeutic and/or preventative immunity” refers to an individual for whom it is desirable to treat, i.e., to prevent, cure, retard, or reduce the severity of influenza disease symptoms, and/or result in no worsening of influenza disease over a specified period of time. Vertebrates to treat and/or vaccinate include humans, apes, monkeys (e.g., owl, squirrel, cebus, rhesus, African green, patas, cynomolgus, and cercopithecus), orangutans, baboons, gibbons, and chimpanzees, dogs, wolves, cats, lions, and tigers, horses, donkeys, zebras, cows, pigs, sheep, deer, giraffes, bears, rabbits, mice, ferrets, seals, whales, ducks, geese, terns, shearwaters, gulls, turkeys, chickens, quail, pheasants, geese, starlings and budgerigars.
One or more compositions of the present invention are utilized in a “prime boost” regimen. An example of a “prime boost” regimen may be found in Yang, Z. et al. J. Virol. 77:799-803 (2002), which is incorporated herein by reference in its entirety. In these embodiments, one or more polynucleotide vaccine compositions of the present invention are delivered to a vertebrate, thereby priming the immune response of the vertebrate to an influenza virus, and then a second immunogenic composition is utilized as a boost vaccination. One or more compositions of the present invention are used to prime immunity, and then a second immunogenic composition, e.g., a recombinant viral vaccine or vaccines, a different polynucleotide vaccine, or one or more purified subunit isolated influenza virus polypeptides or fragments, variants or derivatives thereof is used to boost the anti-influenza virus immune response.
In one embodiment, a priming composition and a boosting composition are combined in a single composition or single formulation. For example, a single composition may comprise an isolated influenza virus polypeptide or a fragment, variant, or derivative thereof as the priming component and a polynucleotide encoding an influenza protein as the boosting component. In this embodiment, the compositions may be contained in a single vial where the priming component and boosting component are mixed together. In general, because the peak levels of expression of protein from the polynucleotide does not occur until later (e.g., 7-10 days) after administration, the polynucleotide component may provide a boost to the isolated protein component. Compositions comprising both a priming component and a boosting component are referred to herein as “combinatorial vaccine compositions” or “single formulation heterologous prime-boost vaccine compositions.” In addition, the priming composition may be administered before the boosting composition, or even after the boosting composition, if the boosting composition is expected to take longer to act.
In another embodiment, the priming composition may be administered simultaneously with the boosting composition, but in separate formulations where the priming component and the boosting component are separated.
The terms “priming” or “primary” and “boost” or “boosting” as used herein may refer to the initial and subsequent immunizations, respectively, i.e., in accordance with the definitions these terms normally have in immunology. However, in certain embodiments, e.g., where the priming component and boosting component are in a single formulation, initial and subsequent immunizations may not be necessary as both the “prime” and the “boost” compositions are administered simultaneously.
In certain embodiments, one or more compositions of the present invention are delivered to a vertebrate by methods described herein, thereby achieving an effective therapeutic and/or an effective preventative immune response. More specifically, the compositions of the present invention may be administered to any tissue of a vertebrate, including, but not limited to, muscle, skin, brain tissue, lung tissue, liver tissue, spleen tissue, bone marrow tissue, thymus tissue, heart tissue, e.g., myocardium, endocardium, and pericardium, lymph tissue, blood tissue, bone tissue, pancreas tissue, kidney tissue, gall bladder tissue, stomach tissue, intestinal tissue, testicular tissue, ovarian tissue, uterine tissue, vaginal tissue, rectal tissue, nervous system tissue, eye tissue, glandular tissue, tongue tissue, and connective tissue, e.g., cartilage.
Furthermore, the compositions of the present invention may be administered to any internal cavity of a vertebrate, including, but not limited to, the lungs, the mouth, the nasal cavity, the stomach, the peritoneal cavity, the intestine, any heart chamber, veins, arteries, capillaries, lymphatic cavities, the uterine cavity, the vaginal cavity, the rectal cavity, joint cavities, ventricles in brain, spinal canal in spinal cord, the ocular cavities, the lumen of a duct of a salivary gland or a liver. When the compositions of the present invention is administered to the lumen of a duct of a salivary gland or liver, the desired polypeptide is expressed in the salivary gland and the liver such that the polypeptide is delivered into the blood stream of the vertebrate from each of the salivary gland or the liver. Certain modes for administration to secretory organs of a gastrointestinal system using the salivary gland, liver and pancreas to release a desired polypeptide into the bloodstream is disclosed in U.S. Pat. Nos. 5,837,693 and 6,004,944, both of which are incorporated herein by reference in their entireties.
In certain embodiments, the compositions are administered into embryonated chicken eggs or by intramuscular injection into the defeathered breast area of chicks as described in Kodihalli S. et al., Vaccine 18:2592-9 (2000), which is incorporated herein by reference in its entirety.
In certain embodiments, the compositions are administered to muscle, either skeletal muscle or cardiac muscle, or to lung tissue. Specific, but non-limiting modes for administration to lung tissue are disclosed in Wheeler, C. J., et al., Proc. Natl. Acad. Sci. USA 93:11454-11459 (1996), which is incorporated herein by reference in its entirety.
According to the disclosed methods, compositions of the present invention can be administered by intramuscular (i.m.), subcutaneous (s.c.), or intrapulmonary routes. Other suitable routes of administration include, but are not limited to intratracheal, transdermal, intraocular, intranasal, inhalation, intracavity, intravenous (i.v.), intraductal (e.g., into the pancreas) and intraparenchymal (i.e., into any tissue) administration. Transdermal delivery includes, but not limited to intradermal (e.g., into the dermis or epidermis), transdermal (e.g., percutaneous) and transmucosal administration (i.e., into or through skin or mucosal tissue). Intracavity administration includes, but not limited to administration into oral, vaginal, rectal, nasal, peritoneal, or intestinal cavities as well as, intrathecal (i.e., into spinal canal), intraventricular (i.e., into the brain ventricles or the heart ventricles), inraatrial (i.e., into the heart atrium) and sub arachnoid (i.e., into the sub arachnoid spaces of the brain) administration.
Any mode of administration can be used so long as the mode results in the expression of the desired peptide or protein, in the desired tissue, in an amount sufficient to generate an immune response to influenza virus and/or to generate a prophylactically or therapeutically effective immune response to influenza virus in a human in need of such response. Administration means of the present invention include needle injection, catheter infusion, biolistic injectors, particle accelerators (e.g., “gene guns” or pneumatic “needleless” injectors) Med-E-Jet (Vahlsing, H., et al., J. Immunol. Methods 171:11-22 (1994)), Pigjet (Schrijver, R., et al., Vaccine 15: 1908-1916 (1997)), Biojector (Davis, H., et al., Vaccine 12: 1503-1509 (1994); Gramzinski, R., et al., Mol. Med. 4: 109-118 (1998)), AdvantaJet (Linmayer, I., et al., Diabetes Care 9:294-297 (1986)), Medi-jector (Martins, J., and Roedl, E. J. Occup. Med. 21:821-824 (1979)), gelfoam sponge depots, other commercially available depot materials (e.g., hydrogels), osmotic pumps (e.g., Alza minipumps), oral or suppositorial solid (tablet or pill) pharmaceutical formulations, topical skin creams, and decanting, use of polynucleotide coated suture (Qin, Y., et al., Life Sciences 65: 2193-2203 (1999)) or topical applications during surgery. Certain modes of administration are intramuscular needle-based injection and pulmonary application via catheter infusion. Energy-assisted plasmid delivery (EAPD) methods may also be employed to administer the compositions of the invention. One such method involves the application of brief electrical pulses to injected tissues, a procedure commonly known as electroporation. See generally Mir, L. M. et al., Proc. Natl. Acad. Sci. USA 96:4262-7 (1999); Hartikka, J. et al., Mol. Ther. 4:407-15 (2001); Mathiesen, I., Gene Ther. 6:508-14 (1999); Rizzuto G. et al., Hum. Gen. Ther. 11:1891-900 (2000). Each of the references cited in this paragraph is incorporated herein by reference in its entirety.
Determining an effective amount of one or more compositions of the present invention depends upon a number of factors including, for example, the antigen being expressed or administered directly, e.g., HA, NA, NP, M1 or M2, or fragments, e.g., M2e, variants, or derivatives thereof, the age and weight of the subject, the precise condition requiring treatment and its severity, and the route of administration. Based on the above factors, determining the precise amount, number of doses, and timing of doses are within the ordinary skill in the art and will be readily determined by the attending physician or veterinarian.
Compositions of the present invention may include various salts, excipients, delivery vehicles and/or auxiliary agents as are disclosed, e.g., in U.S. Patent Application Publication No. 2002/0019358, published Feb. 14, 2002, which is incorporated herein by reference in its entirety.
Furthermore, compositions of the present invention may include one or more transfection facilitating compounds that facilitate delivery of polynucleotides to the interior of a cell, and/or to a desired location within a cell. As used herein, the terms “transfection facilitating compound,” “transfection facilitating agent,” and “transfection facilitating material” are synonymous, and may be used interchangeably. It should be noted that certain transfection facilitating compounds may also be “adjuvants” as described infra, i.e., in addition to facilitating delivery of polynucleotides to the interior of a cell, the compound acts to alter or increase the immune response to the antigen encoded by that polynucleotide. Examples of the transfection facilitating compounds include, but are not limited to inorganic materials such as calcium phosphate, alum (aluminum sulfate), and gold particles (e.g., “powder” type delivery vehicles); peptides that are, for example, cationic, intercell targeting (for selective delivery to certain cell types), intracell targeting (for nuclear localization or endosomal escape), and ampipathic (helix forming or pore forming); proteins that are, for example, basic (e.g., positively charged) such as histones, targeting (e.g., asialoprotein), viral (e.g., Sendai virus coat protein), and pore-forming; lipids that are, for example, cationic (e.g., DMRIE, DOSPA, DC-Chol), basic (e.g., steryl amine), neutral (e.g., cholesterol), anionic (e.g., phosphatidyl serine), and zwitterionic (e.g., DOPE, DOPC); polymers such as dendrimers, star-polymers, “homogenous” poly-amino acids (e.g., poly-lysine, poly-arginine), “heterogeneous” poly-amino acids (e.g., mixtures of lysine & glycine), co-polymers, polyvinylpyrrolidinone (PVP), poloxamers (e.g. CRL 1005) and polyethylene glycol (PEG); and virosomes such as immunopotentiating reconstituted influenza virosome (IRIV). A transfection facilitating material can be used alone or in combination with one or more other transfection facilitating materials. Two or more transfection facilitating materials can be combined by chemical bonding (e.g., covalent and ionic such as in lipidated polylysine, PEGylated polylysine) (Toncheva, et al., Biochim. Biophys. Acta 1380(3):354-368 (1988)), mechanical mixing (e.g., free moving materials in liquid or solid phase such as “polylysine+cationic lipids”) (Gao and Huang, Biochemistry 35:1027-1036 (1996); Trubetskoy, et al., Biochem. Biophys. Acta 1131:311-313 (1992)), and aggregation (e.g., co-precipitation, gel forming such as in cationic lipids+poly-lactide, and polylysine+gelatin). Each of the references cited in this paragraph is incorporated herein by reference in its entirety.
The following materials and methods apply generally to all the examples disclosed herein. Specific materials and methods are disclosed in each example, as necessary.
The practice of the present invention will employ, unless otherwise indicated, conventional techniques of cell biology, cell culture, molecular biology (including PCR), vaccinology, microbiology, recombinant DNA, and immunology, which are within the skill of the art. Such techniques are explained fully in the literature. See, for example, Molecular Cloning A Laboratory Manual, 2nd Ed., Sambrook et al., ed., Cold Spring Harbor Laboratory Press: (1989); DNA Cloning, Volumes I and II (D. N. Glover ed., 1985); Oligonucleotide Synthesis (M. J. Gait ed., 1984); Mullis et al. U.S. Pat. No. 4,683,195; Nucleic Acid Hybridization (B. D. Hames & S. J. Higgins eds. 1984); Transcription And Translation (B. D. Hames & S. J. Higgins eds. 1984); Culture Of Animal Cells (R. I. Freshney, Alan R. Liss, Inc., 1987); Immobilized Cells And Enzymes (IRL Press, 1986); B. Perbal, A Practical Guide To Molecular Cloning (1984); the treatise, Methods In Enzymology (Academic Press, Inc., N.Y.); Gene Transfer Vectors For Mammalian Cells (J. H. Miller and M. P. Calos eds., 1987, Cold Spring Harbor Laboratory); Methods In Enzymology, Vols. 154 and 155 (Wu et al. eds.), Immunochemical Methods In Cell And Molecular Biology (Mayer and Walker, eds., Academic Press, London, 1987); and in Ausubel et al., Current Protocols in Molecular Biology, John Wiley and Sons, Baltimore, Md. (1989). Each of the references cited in this paragraph is incorporated herein by reference in its entirety.
Hemagglutination Inhibition (HAI) Assays
Preimmune and postimmune mouse sera were treated with receptor-destroying enzyme (RDE). HAI antibodies were measured against influenza rgA/Vietnam/1203/2004×A/PR/8/34 influenza (H5N1) vaccine virus. Four HA units of virus were incubated with serial dilutions of RDE-treated mouse sera for at least 30 minutes at room temperature followed by a 30 minute incubation with 0.5% horse erythrocytes. The HAI titer was recorded as the reciprocal of the highest dilution of antisera which inhibits the agglutination of horse erythrocytes.
Viral Micro Neutralization Assays
Influenza vaccine virus rgA/Vietnam/1203/2004×A/PR/8/34 (H5N1) and diluted RDE-treated mouse sera were incubated together at room temperature for 1 hour. The mixture was titrated on monolayers of Madin-Darby canine kidney (MDCK) cells grown in 96-well tissue culture plates. Plates were incubated for 3 days at 37° C. in 5% CO2. At the end of 3 days, the presence of cytopathic effects on cell monolayers was evaluated. Neutralization titers were expressed as the reciprocal of the antibody dilution that completely inhibited virus infectivity in 50% of quadruplicate cultures
Mice, Immunizations and Cell Cultures
HLA DR4 transgenic mice are obtained from C. David (Mayo Clinic) or purchased from Taconic. Non-transgenic H-2b mice are purchased from Charles River Laboratories or other commercial vendors. Immunizations are performed as described in (Ishioka et al., J Immunol, 162(i):3915-25 (1999)). All cells are grown in culture medium consisting of RPMI 1640 medium with HEPES (Gibco Life Technologies) supplemented with 10% FBS, 4 mM L-glutamine, 50 μM 2-ME, 0.5 mM sodium pyruvate, 100 μg/ml streptomycin and 100 U/ml penicillin.
The natural crossreactivity between HLA-DR and IAb can also be exploited to test HTL responses. This evaluation provides an assessment of the antigenicity and immunogenicity of multi-epitope constructs.
HA, HA-PADRE® and PADRE®-HA DNA constructs were designed as follows: the HA sequences were generated by PCR using overlapping complementary oligonucleotides encoding the H5 HA from A/Vietnam/1203/2004 (Accession # AAT73274). The HA sequences were backtranslated using the codon table for Autographa Californica polyhedrovirus. Blocks with 20 nucleotide overlap were annealed together and extended in a gene synthesis reaction (94° C., 30 sec; 58° C., 30 sec; 72° C., 1 min for 5 cycles; 94° C., 30 sec; 72° C., 1 min for 10 cycles) using the proof-reading polymerase Pfu (San Diego, Stratagene). The extended blocks were amplified by PCR (94° C., 30 sec; 58° C., 30 sec; 72° C., 2 min; 30 cycles) to synthesize full-length constructs. The gel purified PCR products were cloned into pFastBac (Carlsbad, Invitrogen) or mammalian vector pMB75.6 and confirmed by sequence analysis. A PADRE® sequence was inserted at a location 5′ or 3′ to the HA DNA sequence into the pFastBac or mammalian PMB75.6 vector, either prior to or subsequent to the cloning of the HA PCR product.
Transgenic mice (HLA-DR4) were injected with 50 III of 1 mg/ml and 0.01 mg/ml of HA, HA-PADRE® and PADRE®-HA DNA constructs in the anterior tibialis muscle of both legs. Mice were immunized two times, one month apart, with bleeds occurring 4 and 2 weeks following primary and secondary immunizations, respectively. ELISA measurements were performed using 96-well, flat-bottom plates (Immunol II, Dynatech, Boston, Mass.) coated with 1 μg recombinant hemagglutinin (Protein Sciences Corporation, Meriden, Conn.). Data are shown as antibody titers determined as the reciprocal of the serum dilution yielding 0.3 OD units (450 nM). Representative results are presented in
In a similar experiment, groups of ten HLA-DR4 transgenic mice were immunized with a dose titration (100 and 10 μg/animal) of PADRE®-HA (SEQ ID NO: 180) and HA (SEQ ID NO:182) DNA vaccines. The mice were immunized three times at 3 week intervals. Two weeks following each immunization, the mice were bled and antibody titers determined by standard ELISA using 0.2 μg purified HA (Protein Sciences) to coat the wells. Antibody titers are given as the reciprocal of the dilution giving an OD reading of 0.3 at 450 nM. Results of specific antibody responses at a high and a low dose in individual animals using HA and PADRE®-HA constructs are shown in
HLA transgenic mouse will serve a valuable tool in evaluating epitope processing and presentation from DNA or viral epitope-based vaccines. These attributes also suggest that the mouse model can be used in influenza challenge studies following vaccination.
The NCBI database was searched for M2e amino acid sequences for representatives of epidemic (H1N1, H3N2), past pandemic (H1N1, H2N2, H3N2) and potential future pandemic (H5N1, H7N7, H9N2) viral strains. As shown in Table 5, a distinct pattern of conserved and varied sequences was observed. Viral strains isolated from humans exhibited the conserved sequence, SLLTEVETPIRNEWGCRCNDSSD (SEQ ID NO:15) which is proposed as a “universal” influenza vaccine. However, potential pandemic strains do not encode this conserved sequence. In contrast, a distinct pattern of sequence variation occurs in viral strains isolated from avian or swine sources, specifically at amino acid positions, 10, 13, 15, 17, and 19. For example, A/Swine/Saskatchewan/18789/02 sequence varies specifically at positions 10 (I→T), position 13 (E→G), position 15 (G→E), position 17 (R→K) and position 19 (N→S) relative to the human-derived sequence. There are other variants but generally with a subset of the same changes.
M2e sequences are cloned into pFastBac (Carlsbad, Invitrogen) or mammalian vector pMB75.6 and confirmed by sequence analysis. A PADRE® sequence is inserted at a location 5′ or 3′ to the M2e DNA sequence into the pFastBac or mammalian PMB75.6 vector, either prior to or subsequent to the cloning of the M2e sequence.
To identify epitopes useful for vaccine design, a multidisciplinary approach is used based initially on amino acid motif searching of viral sequences to identify potential HLA Class II motifs (see Tables 3 and 4). This is followed by high throughput synthetic peptide binding assays using purified HLA molecules to determine affinity and breadth of epitope peptide binding.
Selection of influenza virus strains with potential to initiate pandemics: Influenza virus strains for this study were selected on the basis of host diversity (avian, swine, human), agents of past pandemics (H1N1, H2N2, H3N2) and capacity to cause zoonotic influenza infections of man (H5N1, H1N1, H7N7, H9N2). The selected strains are shown below.
Algorithm motif searches: Motif search algorithms are validated for the most common HLA Class II alleles but will focus on the HLA-DR1 and -DR3 supertypes because we can attain virtually 100% population coverage. The selected influenza viral sequences were scanned for motif positive amino acid sequences using the motif definitions. The peptides specific for DR1 and DR3 supertypes are produced as synthetic peptides.
Selected viral strains with potential to initiate pandemics are as follows:
a)Presence of this symbol (▪) indicates that the gene sequence is available;
b) numerous cases of avian-to-human transmission and fatalities caused by H5N1;
c) The 1968 pandemic was due to a H3N2 virus;
d) The 1957 pandemic was due to H2N2 virus;
e) Classical swine H1N1 virus strain;
f) Isolated from a fatal human case.
Peptide synthesis: The class II peptides are synthesized initially as crude peptides from Mimotopes (Minneapolis, Minn./Clayton, Victoria, Australia) or Pepscan Systems B.V. (Lelystad, Netherlands). These peptides are supplied in small amounts and are typically only 50-70% pure. Larger quantities of selected peptides are synthesized, when needed, using an Applied Biosystems (Foster City, Calif.) 430A peptide synthesizer and fluoronylmethyloxy carbonyl (F-moc) solid phase methods. Peptides synthesized are typically purified to >95% homogeneity by reverse phase HPLC.
In vitro HLA-peptide epitope binding assays: High affinity binding of epitope peptides to HLA molecules is required for immune recognition and has proved to be one of the most highly predictive approaches for identifying epitopes. Capture assays based on the use of the TopCount benchtop microplate scintillation counter (Packard Instruments) allow the high throughput, sensitivity and compatibility with data automation platforms.
HLA Class II purification: The binding assay requires the use of purified HLA Class II molecules. A large number of different types of cells are available including EBV-transformed homozygous human B cell lines, mouse B cell lymphomas or mastocytomas, transfected fibroblasts or single MHC allele transfected 721.221 lines. HLA molecules are purified from cell lysates using monoclonal antibody-based affinity chromatography.
Measurement of peptide binding to HLA molecules and data analysis: The binding assay to be utilized is a competitive system that is based on the use of known 125I radiolabeled peptide ligands112. To determine the IC50 of peptide binding, the concentration of test peptide yielding 50% inhibition of the binding of the radiolabeled peptide is calculated. Typical test concentrations range from 120 μg/ml-120 pg/ml. Under the conditions utilized, the measured IC50 values are reasonable approximations of the Kd values.
Epitopes that are naturally processed and presented to the immune system using peptides are identified as high affinity binders to HLA molecules and peripheral blood mononuclear cells (PBMC) from normal human donors and HLA transgenic mice. It is necessary to address epitope immunogenicity because not all motif positive peptides are immunogenic nor is it likely that all epitopes are generated equally during infection. Typically two methods to document epitope immunogenicity and utility are used; 1) in vitro assays using PBMC from normal donors and 2) immunization studies with HLA transgenic mice. Recognition of epitope peptides by human PBMC in a recall assay is the most direct method to verify the authenticity of an epitope because responses demonstrate the epitope was generated as the course of natural infection and that the needed T-cell receptor (TCR) repertoire exists. Finally, the HLA transgenic mouse is well suited for testing vaccine constructs because the proteosome processing preferences and TCR repertoires of mice overlap significantly with humans.
Assay for recall memory influenza responses using human PBMC: Based on preliminary data presented, past studies44, and those of others42,43,45, responses to multiple epitopes are expected because the selection process is for immunologically conserved epitopes. The assays detecting IFN-γ are performed as described above and according to manufacturers' protocols.
It has been demonstrated that CD4+ cells can promote survival to a lethal dose of influenza infection. The mechanisms that may be involved are several including their classic contribution as helpers during the generation of flu-specific CD8+ CTL and antibody producing B cells. Potentially, CD4+ cells following influenza infection may have an effector function and directly mediate viral clearance by IFN-γ-dependent mechanisms and/or by direct cytolytic effects on infected cells. Accordingly, HTL activity is measured as a function of IFN-γ secretion by CD4+ T-lymphocytes, again using an ELISPOT assay as described. Depending on the results obtained using IFN-γ as a readout, IL-2 or TNF-γ could also be assayed using an ELISPOT format.
A collection of positive and control peptides for each supertype are required to ensure the specificity of the influenza-specific responses. Defined epitopes from various pathogens, generally HIV, HBV, HCV and Plasmodium falciparum can be used as negative controls assuming that the donors have not been exposed. Positive control peptides are usually derived from HCMV, EBV, and influenza. Negative and positive control peptides to be used for each supertype are identified from previous studies and the literature.
Human M2e-specific memory B cells using a novel ELISPOT system are identified. This assay has been used to demonstrate that the anthrax vaccine (AVA: BioThrax) elicits a substantial population of protective-antigen specific memory B cells144. The assay relies on a 6 day polyclonal [pokeweed mitogen extract (ICN), fixed S. aureus, Cowan (Sigma)] stimulation of PBMC followed by an antigen-specific ELISPOT for detection of memory B cells that have differentiated into antibody secreting cells. Specifically, 96-well filter plates (Millipore) are coated with M2e peptide followed by addition of activated PBMC. After an incubation period, the plates are subsequently washed and incubated in the presence of mouse anti-human pan IgG Fc biotin conjugated antibody (Hybridoma Reagent Laboratory). Following washing, the plates are incubated with HRP-conjugated avidin-D (Vector Laboratories) and developed using AEC (Sigma). Controls for the assay includes a non-M2e antigen negative control, such as KLH (Pierce), and a positive control which consists of detection of all IgG secreting cells by coating the plate with goat anti-human Ig. Data are expressed as frequency of M2e-specific B cells as a percentage of the total IgG+ memory B cells/106 PBMC. Poke weed mitogen (PWM) is assayed for activity. Individual lots of PWM are titrated for activity before use. It should be noted that although the M2e epitope is highly conserved, there are sequence variations that must be addressed. For example, the most conserved sequence of the human influenza A viruses is SLLTEVETPIRNEWGCRCNDSSD (SEQ ID NO:15). However, Shiver and colleagues have reported that antibodies induced by this sequence do not cross-react on M2 peptides derived from the pathogenic H5N1 virus54. The A/Hong Kong/483/97 has multiple sequence differences noted as underlined, SLLTEVETLTRNGWGCRCSDSSD (SEQ ID NO:209). If the M2e B cell epitope is to be used as a pandemic vaccine component then sequences from appropriate strains with a potential to initiate pandemics will need to be considered. Various influenza strains indicated in Table 5 were aligned and examined for sequence variation in the M2e epitope. Four different strains, as shown in Table 6, demonstrated sequence variation. Peptides corresponding to these strains are synthesized and used to immunize mice. Each M2e-specific antibody response induced is evaluated for the capacity to bind the four different sequences.
Immunogenicity testing of HTL and B cell epitopes in HLA transgenic and non transgenic mice: HLA-DR4 transgenic mice from Taconic, a commercial source are also utilized. Additionally, mice of the b haplotype, e.g., C57B1/6 are utilized, to evaluate the immunogenicity of HLA-DR-restricted peptides67,139. The rationale for using b haplotype mice is based on the observation that the motifs recognized by DR alleles often cross-react on murine class II alleles. Immunogenicity of test epitopes are generally accomplished by immunizing mice with pools of peptides (5-10) emulsified in IFA (for CTL) and CFA (for HTL) followed by in vitro testing of splenocytes 14 days later for epitope-specific T lymphocyte responses.
Construction and Testing of HTL Epitope Strings:
Epitope strings encompassing 1-10 different HTL epitopes under the control of a single promoter are synthesized and incorporated into a standard plasmid, pcDNA 3.1 (Invitrogen, San Diego). To facilitate testing and optimization, each set of epitopes for a given construct is chosen to provide a balanced representation of epitopes which are already known to be immunogenic in IAb mice. In addition, all the peptides corresponding to junctions are synthesized and tested for binding to IAb and, most importantly, for binding to a panel of fourteen different DR molecules, representative of the most common DR alleles worldwide (Southwood et al., J Immunol, 160(7):3363-73 (1998)). Thus, HTL epitopes that are not directed to an antigen of interest are not created within these plasmids. However, should junctional regions with good DR binding potential (and hence, potential DR restricted immunogenicity in vivo) be detected, a spacer such as GPGPG is introduced to eliminate them. In all constructs, the number of Class I junctional motifs will also be minimized.
Experimental vaccine plasmids are tested for immunogenicity using HLA DR transgenic mice and/or mice of the H2b haplotype. Proliferation and/or cytokine production are measured (IL5, IFNγ). In a typical protocol, cardiotoxin treated mice are injected i.m. with 100 μg of each plasmid and responses evaluated eleven days later (Ishioka et al., J Immunol, 162(7):3915-25 (1999)).
Since the ultimate use of optimized constructs is a human vaccine, optimized human codons are utilized. However, to facilitate the optimization process in HLA transgenic mice, care are applied to select, whenever possible, human codons that are also optimal for mice. Human and murine codon usage is very similar. See, e.g., Codon usage database at http://www.kazusa.or.jp/codon/.
Human cells transfected with the various multi-epitope nucleic acid vaccine constructs can be used in antigenicity assays, conducted in parallel with in vivo testing in HLA transgenic mice. Any potential discrepancy between multi-epitope nucleic acid vaccine efficacy, due to the differential codon usage, is addressed by the availability of these two different assay systems.
Typically, antigenicity and immunogenicity testing of plasmid constructs is conducted in parallel. In vivo testing in transgenic mice are performed for A2, A11, and B7 HLA transgenic mice. Following a standard protocol, cardiotoxin pretreated mice are injected i.m. with 100 μg of each plasmid and responses evaluated eleven days later (Ishioka et al., J Immunol, 162(7):3915-25 (1999)). Assays will include ELISPOT from freshly isolated cells, as well as interferon gamma release. All of the above mentioned techniques are well established in the art. The simultaneous measurement of responses against epitopes is not problematic, as large colonies of transgenic mice are established for these HLA types. Groups of four to six mice are adequate to measure responses against six to ten different epitopes, in multiple readout assays.
Testing for Interactions Between PADRE®, HA, M2e sequences and HTL Epitopes
The activities described above yield small, functional blocks of epitopes, which are utilized to demonstrate simultaneous responses/antigenicity against all epitopes analyzable. These blocks are the subject to further optimization. Using these same constructs, immunodominance is assessed. The results obtained with the pool of constructs are then compared with the results obtained with the same construct, injected separately.
Primary interferon-gamma (IFN-γ) ELISPOT (enzyme linked immunospot) assay was used to identify candidate vaccine epitopes. Peripheral blood mononuclear cells (PBMCs) were collected by leukapheresis from healthy human donors. The PBMCs were purified using standard Ficoll-Paque (Amersham) density gradient centrifugation and subsequently frozen at 5×107 cells per ml. PBMCs were thawed and were either rested for 5 days (no peptide) or stimulated for 7 days with the appropriate peptides at 37° C. in media at 2.5×106 cells per mL. Elispot plates (Millipore IP plate) were coated with anti-human IFN-γ antibody clone 1-D1K (Mabtech, Cat# 3420-3, 1 mg/mL) and incubated overnight at 4° C. The following day, PBMCs were depleted of CD8+ cells using human DYNAbeads (DYNAL Biotec Cat# 111.47, OSLO, Norway). The depleted PBMCs with enriched CD4+ cells were then plated onto ELISPOT plates previously blocked with RPMI 1640 containing 10% FCS. Irradiated PBMCs coated with peptide were added to the plated PBMCs and the plates were incubated at 37° C. for 20 hours. The next day the plates were incubated with biotinylated mouse anti-human IFN-γ antibody and developed with Vectastain Elite Vector Cat# PK-6100 according to manufacturer's instructions. The spots were counted on an ELISPOT counter (AID). Donors were considered positive for a peptide if the number of spots was over 3 times background as determined by responses to irrelevant peptides (non influenza). Representative results are shown in FIGS. 3A-B.
In another experiment, frozen Donor PBMC were thawed and rested overnight in media containing RPMI 5% AB human serum/complete media followed by a five day expansion of peptide-specific HLA-DR-restricted HTL using a pool of approximately 10 peptides (1 μg/ml final concentration of each peptide). On day five, CD4+ T cells were enriched by removing CD8+ T cells using Dynal beads and a standard IFNγ ELISPOT performed. Negative control peptides (HIV, HCV) were used to determine background responses. Results for donor 753, 6018, 716, AC08 and AC02 are shown in
In another experiment, frozen Donor PBMC were thawed and rested five days in media containing RPMI 5% AB human serum/complete media. On day five, CD4+ T cells were enriched by removing CD8+ T cells using Dynal beads and a standard IFNγ ELISPOT performed. Negative control peptides (HIV, HCV) were used to determine background responses. Results for donor 3501 are shown in
The Human influenza epitope-specific immune responses can be summarized as follows:
A universal spacer consisting of GPGPG was developed to separate HTL epitopes, thus disrupting junctional epitopes. The logic behind the design of this spacer is that neither G nor P are used as primary anchors, positions 1 and 6 in the core region of an HTL peptide epitope, by any known murine or human MHC Class MHC Class II molecule. The gap of five amino acids introduced by this spacer separates adjacent epitopes so the amino acids of two epitopes cannot physically serve as anchors in the 1 and 6 positions. The utility of the GPGPG spacer is tested using synthetic peptides composed of IAb.
The ability of multi-epitope HTL DNA-based constructs to induce an HTL response in vivo is evaluated by intramuscular immunization of H2bxd mice with an EP-HIV-1043-PADRE® construct. Eleven days after immunization, no booster immunizations were administered, CD4 T cells are purified from the spleen, and peptide specific HTL responses are measured in a primary γ-IFN ELISPOT assay. Overall, the HTL responses induced by DNA immunization with the multi-epitope influenza HTL construct are generally of equal or greater magnitude than the responses induced by peptide immunization.
Thus, as described above, the invention provides a novel method and system for automatically analyzing polypeptide junctions, eliminating or reducing the number of junctional epitopes, and identifying spacer combinations to optimize the efficacy of multi-epitope constructs. Those skilled in the art will know, or be able to ascertain using no more than routine experimentation, many equivalents to the specific embodiments of the invention described herein. These equivalents are intended to be encompassed by the following claims.
Constructs are designed based on computer programs to optimize proteosomal processing and minimize junctional epitopes: Strategies have been developed to optimize epitope processing efficiency from multi-epitope genetic constructs and to minimize the generation of neo-epitopes generated at the junction of epitopes which may divert the immune responses from the specified desired epitopes67,69. The incorporation of preferred flanking amino acids to optimize proteosomal processing and a motif searching function is performed using a computer program.
DNA Vaccine production: DNA vaccine production is performed using routine methods based on primer extension with overlapping oligonucleotide PCR primers, averaging 70 nucleotides in length with 15 nucleotide overlaps58. The synthetic gene encoding the epitopes is cloned into the clinically accepted pMB75.6 vaccine backbone145.
The influenza virus vaccine is formulated in various test adjuvants as described above. Other vaccine delivery formats are also utilized including DNA, AlphaVax viral vaccines and virosomes, and in particular IRIVs.
Assessment of vaccine immunogenicity: Immunogenicity testing is performed primarily using the HLA-DR4 transgenic mice from Taconic and CB6F1 (b×d haplotype) mice to measure responses specific for the influenza-derived HTL epitopes and HA-specific antibodies. Immunogenicity evaluation in mice is a useful tool to assess efficient antigen processing and epitope presentation specifically for the vaccine construct. The spacers adjacent to epitopes that are found to be suboptimally immunogenic in a vaccine construct can be modified, through site-directed mutagenesis, in one or more cycles of secondary optimization.
B-cell assays evaluating vaccines encoding or containing the B cell epitope M2e: An ELISA-based assay measuring antibodies specific for the M2e sequence are performed. M2e, the external domain of the transmembrane viral M2 protein, is highly conserved amongst various influenza strains of differing subtypes. Groups of 10 C57B1/6, CB6F1, or DR4 transgenic mice are immunized with a dose titration of PADRE®-M2e peptide, 0.1, 1, 10 μg adsorbed to 250 μg of alum (Superfos Biosector) as an example of an adjuvant suitable for humans. Alternatively, the PADRE®-M2e immunogen may be DNA. Vaccines are administered in volumes of 100 μl, two or three times at 3-4 week intervals by s.c. injection at the base of the tail. Blood samples are obtained prior to immunizations and at monthly intervals. To determine antibody titers, a standard ELISA assay are performed using 96-well Immunol II plates coated with 0.1 μg/well of the B cell epitope. As a control, mice are immunized with the B cell epitope adsorbed to alum (not linked to PADRE®). The protective capacity of the M2e-specific antibody responses are measured in the viral challenge experiments described below.
Augmentation of HA-derived HTL and antibody responses using DNA vaccines followed by HA protein immunization: Prior immunization with conserved influenza virus HTL epitopes will augment HTL and antibody responses induced using protein-based or inactivated virus-based vaccines. HLA transgenic mice are initially immunized separately or in a prime-boost format using the DNA, and peptides in adjuvant vaccines. These immunizations are followed by inoculation with various HA proteins (0.1, 1, 10 μg/mouse). The HTL and antibody responses are measured (as described above) and directly compared to mice receiving only the conventional HA vaccines. Purified baculovirus-expressed recombinant HA proteins (Protein Sciences, Inc, Meriden, Conn.) corresponding to A/Hong Kong/156/97 (H5) and A/Hong/Kong/1073/99 (H9) are used. The rationale for using H5 and H9 proteins is due to their pandemic potential as observed by transmission of these variants from avian to human18,146.
The efficacy of vaccines composed of conserved influenza HTL and B cell epitopes are evaluated in an influenza viral challenge mouse model. For example, peptides are formulated in various adjuvants and tested for immunogenicity. If a particular adjuvant is superior in augmenting cellular and humoral responses then this adjuvant is used in the challenge studies. Initially, protection against various divergent influenza subtypes is determined by immunizing mice separately with selected DNA, peptides in adjuvant, HA proteins, inactivated and live attenuated vaccines. Doses and immunization schedules are determined according to the immunogenicity studies described above. The capacity of the influenza HTL and B cell epitope-based vaccines to afford protection is compared to the HA protein, inactivated and live attenuated vaccines. Finally, the HA protein combined with the DNA, and peptides in adjuvant vaccines using heterologous prime boost immunization schemes are evaluated for protection. Additionally, emphasis is placed on validating an immunization strategy that induces a protective immune response in the shortest amount of time which is likely an important factor to consider in the event of a pandemic influenza occurrence.
Murine influenza challenge models. Viral challenge studies are performed as previously described75,147,148. Initially, mice are immunized with selected vaccines or combinations using doses and immunization schedules that are most immunogenic. To determine the level of protection afforded by the various immunization strategies, immunized mice are challenged with various subtypes of influenza viruses that differ in virulence for mice including human viruses as well as avian and viruses with pandemic potential. Using a number of different subtypes will evaluate the level of protective broadly cross-reactive immunity induced by immunization of mice with the various vaccines expressing conserved HTL epitopes. The following are examples of subtypes for challenge studies: mouse adapted A/Taiwan/1/86 (H1N1); mouse-adapted A/Ann Arbor/6/60 (H2N2); mouse-adapted A/Philippines/1/82 (H3N2); highly pathogenic avian A/Hong Kong/483 (H5N1); a recent human isolate A/Hong Kong/213/03 (H5N1); A/Hong Kong/1073/99 (H9N2); and an H7N7 strain.
The 50% mouse infectious dose (MID50) and 50% lethal dose (LD50) titers are determined for the C57B1/6 mouse strain. Groups of 10-20 mice are lightly anesthetized and infected intranasally (i.n.) with approximately 100-1,000 MID50 of virus. Three and six days post-infection, 5 mice per group are sacrificed and multiple organs including nasal turbinates, lungs and brains are collected and titered in embryonated eggs or MDCK cells for the presence of infectious virus. For viruses that cause lethal disease, and additional group of ten mice are monitored for weight loss and survival over a period of 14 days post-infection.
The use of conserved HTL epitopes delivered by peptides in adjuvant and DNA viral vehicles are used to generate a protective vaccine against influenza.
The effect of PADRE® on immunogenicity was also analyzed by measuring antibody function. Antibodies in the immune sera from PADRE®-HA and HA immunized mice described in Example 2 and shown in
Hemagglutination inhibition (HAI) is a standard technique used to evaluate HA-specific antibody responses following immunization or infection. The assay is dependent on the ability of the anti-HA antibody to inhibit the interaction between viral HA and erythrocyte sialic acid. In these experiments, pre-immune and post-immune mouse sera were treated with receptor-destroying enzyme (RDE). HAI antibodies were measured against influenza rgA/Vietnam/1203/2004×A/PR/8/34 influenza (H5N1) vaccine virus. Four HA units of virus were incubated with serial dilutions of RDE-treated mouse sera for at least 30 minutes at room temperature followed by a 60-minute incubation with 1% horse erythrocytes. The HAI titers are recorded as the reciprocal of the highest dilution of antisera which inhibited the agglutination of horse erythrocytes. Typically, immune ferret sera are used as a positive control and naïve mouse sera for the negative control. While only 3/10 animals exposed to HA induced antibodies capable of inhibiting hemagglutination, (20, 40 and 80 titer), 5/10 animals exposed to PADRE®-HA induced antibodies capable of inhibiting hemagglutination (20, 20, 20, 80 and 160 titer).
The Micorneutralization assay also used influenza vaccine virus rgA/Vietnam/1203/2004×A/PR/8/34 influenza (H5N1). The virus and diluted RDE-treated mouse sera were incubated together at room temperature for 1 hour. The mixture was titrated on monolayers of Madin-Darby canine kidney (MDCK) cells grown in 96-well tissue culture plates. After an overnight incubation, the cells were fixed and the presence of influenza A NP protein in infected cells was detected by ELISA as described in the WHO Animal influenza manual. Detection of NP protein in infected cells is more sensitive than scoring viral cytopathogenicity. Typically, immune ferret sera are used as a positive control and naïve mouse sera for the negative control. While none of the animals exposed to HA induced positive viral neutralization responses, 2/10 animals exposed to PADRE®-HA induced positive viral neutralization responses (160 and 640 titer).
The results of these experiments, as summarized in
Groups of ten HLA-DR4 transgenic mice were immunized with either PADRE®-HA (SEQ ID NO:174) or HA (SEQ ID NO:185) recombinant protein. The proteins were delivered using alum as an adjuvant. The mice were immunized with a dose titration (10 and 1 μg of recombinant protein/animal) three times at 1 month intervals. Two weeks following each immunization, the mice were bled and antibody titers determined by standard ELISA using 0.2 μg purified HA (Protein Sciences) to coat the wells. Representative results are shown in
Groups of ten HLA-DR4 transgenic mice were immunized with either PADRE®-HA (SEQ ID NO:174) or HA (SEQ ID NO:185) recombinant protein. The proteins were delivered using alum and Provax™ as an adjuvant. The mice were immunized with a dose titration (1 and 0.1 μg of recombinant protein/animal) two times at 1 month intervals. Two weeks following each immunization, the mice were bled and antibody titers determined by standard ELISA using 0.2 μg purified HA (Protein Sciences) to coat the wells. Representative results are shown in
156. Stevens, J et al, 2006, “Structure of the uncleaved human H1 hemagglutinin from the extinct 1918 influenza virus,” Science 312:404.
—indicates binding affinity > 10,000 nM.
This application claims priority to provisional application 60/838,859, filed Aug. 21, 2006 and to provisional application 60/801,065, filed May 18, 2006, each of which is herein incorporated by reference.
| Number | Date | Country | |
|---|---|---|---|
| 60801065 | May 2006 | US | |
| 60838859 | Aug 2006 | US |
