Patent Application
20130295131
Virus like particle (VLP) vaccines are recombinant structures that mimic the overall structure of virus particles and exhibit adjuvant properties capable of inducing neutralizing immune responses. VLPs have been used successfully to protect humans from hepatitis B virus and human papillomavirus infection. A number of VLP platforms have been engineered to display a range of antigens on their surface and are currently being explored for their potential to combat other infectious diseases and cancer.
VLP technology has the potential to allow rapid evaluation of large numbers of candidate antigens, provided such engineered VLP systems are sufficiently adaptable to display the antigens, either alone or in various combinations, with minimal groundwork.
Various VLP platforms are based on viral proteins that can self-assemble without the infectious viral nucleic acid component. Other platforms display heterologous antigenic components directly on the surface of intact virus particles that contain infectious or partially infectious nucleic acid components. Such particles are viral in nature, and are aptly described as modified virus particles, but are also described herein as VLPs because they are typically recombinant and can be used to display heterologous antigens. VLP technologies that involve genetic fusion of antigens to virus coat proteins (CP) and are typically limited to small peptide antigens. Often, the antigens displayed in those systems negatively affect virus particle formation and recovery. This high degree of unpredictability requires that an individualized program of sequence modification, expression analysis, and purification process development must first be carried out for each antigen prior to conducting even preliminary immunological studies.
Method are described for generating virus-like particles linked to antigens through protein-protein interaction.
In one embodiment, a method of generating a virus-like particle covalently linked to a polypeptide of interest is presented comprising: providing a first polypeptide fused to viral coat protein, and providing a second polypeptide fused to the polypeptide of interest, wherein the first polypeptide and the second polypeptide are capable of protein-protein interaction such that covalent links are formed between the first and second polypeptides via oxidative cross-linking, and wherein the viral coat protein is capable of assembling into a virus-like particle.
In another embodiment, a method of generating a multivalent virus-like particle covalently linked to two or more polypeptides of interest is presented comprising: providing a viral coat protein comprising a Carboxy-terminal fusion with the amino acid sequence TEFCA, and providing two or more different polypeptides of interest individually fused to InaD or a fragment of InaD containing the PDZ1 domain, wherein the TEFCA sequence and the PDZ1 domain are capable of protein-protein interaction such that covalent links are formed via oxidative cross-linking, and wherein the viral coat protein is capable of assembling into a virus-like particle, whereby a multivalent virus-like particle is formed.
In yet another embodiment, a vaccine is described comprising: a first polypeptide fused to viral coat protein, and a second polypeptide fused to an antigen of interest, wherein the first polypeptide and the second polypeptide are capable of protein-protein interaction such that covalent links are formed between the first and second polypeptides via oxidative cross-linking, and wherein the viral coat protein is assembled into a virus-like particle, such that the antigen is displayed on the virus-like particle.
The following detailed description is of the best currently contemplated modes of carrying out exemplary embodiments of the invention. The description is not to be taken in a limiting sense, but is made merely for the purpose of illustrating the general principles of the invention, since the scope of the invention is best defined by the appended claims.
Broadly, an embodiment of the present invention generally is a method for generating virus-like particles (VLPs) that can display other proteins through covalent protein-protein linkages.
The instant approach helps to overcome many of the shortcomings of traditional VLP production methodologies by separating manufacturing of the VLP scaffold from antigen production. Consequently, testing of new antigens in a VLP format may only require production of the antigenic component.
Large quantities of the universal VLP antigen acceptor scaffold can be produced, eliminating the need for complicated and time-consuming work with recombinant virus constructs. When brought together, the scaffold and recombinant antigens can spontaneously associate and covalently lock together to form mature VLP particles with high-density surface arrays of antigen. For testing new antigens, they can be expressed with a small linkage moiety, and then be mixed with the universal scaffold to form the antigen-specific VLPs.
An important aspect of this approach can be in the mechanism of linkage that is used to associate the coat protein with the antigen protein. Kimple, Siderovski, and Sondek (EMBOJ 20(2001)4414-4422) observed that the N-terminal PDZ domain of InaD could interact with, and covalently bind to, the C-terminal five amino acid sequence of NorpA. Kimple and Sondek went on to describe how that interaction could be used for protein affinity purification and labeling for biochemical detection (BioTechniques 33(2002)578-590; U.S. Pat. No. 7,309,575). However, they did not contemplate the use of this type of linkage for VLP vaccine production.
In another embodiment of the instant invention, other protein pairs may covalently interact in a similar way and may be used to generate VLPs displaying antigens. In the interaction between SITAC and the Tetraspanin L6 Antigen, described by Borrell-Pages, et al., (MolBiolCell 11(2000)4217-4225), covalent interaction is likely but it is less well-characterized than the InaD/NorpA interaction.
In another embodiment of the instant invention it is contemplated that the sequences of the interacting protein domains can be modified to adjust the degree of affinity. Such modifications may be achieved through rational design (for example, see Wedemann et al. J Mol Biol 343(2004)703-718), or through mutation and optimization (see, for example, U.S. patent application Ser. No. 10/637,758, herein incorporated by reference in its entirety).
In another embodiment of the instant invention it is contemplated that any protein capable of forming a VLP, can be decorated with one or more proteins or peptides of interest through the covalent protein-protein interactions described herein.
The interaction between the NorpA peptide and InaD was used to mediate covalent interactions between coat protein in intact virus particles and other proteins. For these experiments, the gene sequence encoding the C-terminal pentapeptide (TEFCA, SEQ ID NO: 01) of NorpA was fused to the gene encoding the Tobacco Mosaic Virus (TMV) U1 strain coat protein such that the resultant coat protein (CP) contained a C-terminal extension of the TEFCA (SEQ ID NO: 01) amino acid sequence. The InaD moiety was produced using a TMV-based plant viral vector system in various fusion configurations with the green fluorescent protein (GFP) and/or a poly-histidine tag.
The reducing environment of the cytosol of cells producing either the InaD or NorpA protein fragments can be expected to minimize unwanted crosslinking between the unpaired cysteines of the each protein during expression. Upon lysis, however, the contents of the cells can be released into a potentially oxidative environment, so the presence of anti-oxidants and/or reducing agents during extraction can be useful to facilitate recovery of the protein or virus in an unoxidized and soluble state.
Recombinant virus preparations representing multiple configurations of viral coat protein with a C-terminal TEFCA (SEQ ID NO: 01) sequence were produced. The amino acid sequences of the coat protein-TEFCA fusion for two such preferred constructs, U1CP_TEFCA_Direct and U1CP_TEFCA_Spacer, are shown in
The covalent linkage between U1CP_TEFCA_Spacer and IGH is based on oxidative cross-linking between unpaired cysteines that are brought into juxtaposition by docking of the TEFCA (SEQ ID NO: 01) peptide with InaD domain as diagrammed in
When the polyhistidine-tagged InaD protein was incubated with the TEFCA-modified virus, similar evidence of covalent linkage between the proteins was observed. Moreover, the covalent complexes could be precipitated with 4% polyethylene glycol (MW 8,000) that is used to precipitate viruses, indicating that TEFCA-modified virus particles had been decorated with the InaD protein.
This approach can provide important advantages for VLP technology. Typical approaches to create VLP vaccines often do not accommodate whole proteins, and are based on genetic fusions of antigenic peptides in various positions within the coat protein. Coat proteins with genetic fusions to peptides frequently impair virion assembly or cause other anomalies that can lead to low virion recovery or encouragement of genetic instability leading to loss or change of the sequences encoding the peptide. Other strategies for production of VLPs that display foreign epitopes often require bifunctional chemical cross-linking reagents, or are based on non-covalent interactions between the proteins mediated by avidin:biotin or similar interactions. Those non-covalent interactions, though stable on a timescale of hours to days, may not be sufficiently stable during the time period of days, weeks, or months that may be required for storage prior to their use as immunogens.
This interaction described herein is specific and covalent and can mediate linkage of the antigen protein to the virus-based VLP scaffold to form VLPs decorated on their surface with high concentrations of antigen. Mixtures of various antigens or other molecules, including immunomodulatory agents such as cytokines or toll-like receptor agonists fused to the InaD domain can also be bound to the VLP scaffold to create multivalent VLP particles (
In addition to displaying protein antigens on the virus particle surface, the instant system can also be useful for instances where it is desirable to decorate the particle surface with proteins such as enzymes and antibodies for applications in which high-density protein arrays are important, such as for biocatalyst and biosensor applications.
NorpA C-terminal amino acid sequence:
InaD fragment (13-107):
Tetraspanin L6 antigen:
SITAC18:
It should be understood, of course, that the foregoing relates to exemplary embodiments of the invention and that modifications may be made without departing from the spirit and scope of the invention as set forth in the following claims.
This application claims priority from U.S. Provisional Application No. 61/258,152, filed Nov. 5, 2009. The prior application is hereby incorporated by reference in its entirety.
| Filing Document | Filing Date | Country | Kind | 371c Date |
|---|---|---|---|---|
| PCT/US10/55717 | 11/5/2010 | WO | 00 | 5/3/2013 |
| Number | Date | Country | |
|---|---|---|---|
| 61258152 | Nov 2009 | US |
