The present application is a National Stage application of International Application No. PCT/CN2019/089940, filed Jun. 4, 2019, which is based on and claims the benefit of priority from Chinese application No. 201810563504.2, filed on Jun. 4, 2018, the disclosures of both of which are incorporated herein by reference in its entirety.
The instant application contains a Sequence Listing which has been submitted electronically in ASCII format and is hereby incorporated by reference in its entirety. Said ASCII copy, created Dec. 1, 2020, is named IEC180089_seq1_EN and is 98,304 bytes in size.
The invention relates to the field of molecular virology and immunology. In particular, the invention relates to a mutated HPV66 L1 protein (or a variant thereof), a sequence encoding the same, a method for preparing the same, and a virus-like particle comprising the same, wherein the protein (or a variant thereof) and the virus-like particle can induce the generation of neutralizing antibodies against at least two HPV types (e.g. HPV66 and HPV56, or HPV66, HPV56 and HPV53), and therefore can be used to prevent infection by said at least two HPV types, and a disease caused by said infection, such as cervical cancer and condyloma acuminatum. The invention further relates to the use of the protein and the virus-like particle in the manufacture of a pharmaceutical composition or a vaccine for preventing infection by said at least two HPV types, and a disease caused by said infection, such as cervical cancer and condyloma acuminatum.
Human Papillomavirus (HPV) mainly causes warts in skin and mucosa. HPV types are divided into high-risk types and low-risk types depending on their association with tumorigenesis. Among them, infection by high-risk HPV types has been demonstrated to be the leading cause of genital cancer including cervical cancer in women; and low-risk HPV types mainly cause condyloma acuminatum. The most effective way to prevent and control HPV infection is to vaccinate HPV vaccines, particularly vaccines against high-risk HPV types causing cervical cancer.
Major capsid protein L1 of HPV has the characteristic of self-assembling into hollow Virus-Like Particle (VLP). HPV VLP has a symmetrical icosahedral structure composed of 72 pentamers of major capsid protein L1 (Doorbar, J. and P. H. Gallimore. 1987. J Virol, 61(9): 2793-9). HPV VLP is highly similar to natural HPV in terms of structure, retains most of the neutralizing epitopes of natural virus, and can induce the generation of high-titer neutralizing antibodies (Kirnbauer, R., F. Booy, et al. 1992 Proc Natl Acad Sci USA 89(24): 12180-4).
However, the existing studies show that HPV VLPs mainly induce the generation of neutralizing antibodies against the same HPV type, produce the protective immunity against the same HPV type, and only have low cross-protective effect among a few highly homologous HPV types (Sara L. Bissett, Giada Mattiuzzo, et al. 2014 Vaccine. 32:6548-6555). Therefore, the existing HPV vaccines have a very limited protection range. In general, VLP of one HPV type can only be used to prevent infection by the same HPV type. In this case, if it needs to broaden the protection range of HPV vaccines, the only way is to add VLPs of more HPV types in vaccines. Currently, the commercially available HPV vaccines, including Gardasil® from Merck (which is a quadrivalent vaccine against HPV16, 18, 6 and 11), Cervarix® from GSK (which is a bivalent vaccine against HPV16 and 18), and Gardasil®9 from Merck (which is a 9-valent vaccine against HPV6, 11, 16, 18, 31, 33, 45, 52 and 58), are prepared by combining VLPs of multiple HPV types. However, such a solution would greatly increase the production cost of HPV vaccines, and might cause safety problem due to an increase in immunizing dose.
Therefore, it is urgent in the art to develop HPV virus-like particles capable of inducing the generation of protective neutralizing antibodies against multiple HPV types, so as to prevent infection by multiple HPV types, and a disease caused by the infection, such as cervical cancer and condyloma acuminatum, more economically and effectively.
Contents of Invention
The invention is at least partially based on the inventors' surprising discovery: after substitution of a specific segment of L1 protein of Human Papillomavirus (HPV) Type 66 with the corresponding segment of L1 protein of a second HPV type (such as HPV56), the mutated HPV66 L1 protein thus obtained can induce the generation of high-titer neutralizing antibodies against HPV66 and the second HPV type (such as HPV56) in organisms, and its protection effect is comparable to that of a mixture of HPV66 VLP and VLP of the second HPV type, its protection effect against HPV66 is comparable to that of HPV66 VLP alone, and its protection effect against the second HPV type (such as HPV56) is comparable to that of the VLP of the second HPV type alone.
In addition, based on the substitution above, other one or two specific segments of HPV66 L1 protein can be further substituted with the corresponding segment of L1 protein of a third HPV type (such as HPV53), and the mutated HPV66 L1 protein having double substitutions thus obtained can induce the generation of high-titer neutralizing antibodies against HPV66, the second HPV type (such as HPV56) and the third HPV type (such as HPV53); and its protection effect is comparable to that of a mixture of HPV66 VLP, VLP of the second HPV type and VLP of the third HPV type, its protection effect against HPV66 is comparable to that of HPV66 VLP alone, its protection effect against the second HPV type (such as HPV56) is comparable to that of the VLP of the second HPV type alone, and its protection effect against the third HPV type (such as HPV53) is comparable to that of the VLP of the third HPV type alone.
Therefore, in an aspect, the invention provides a mutated HPV66 L1 protein or a variant thereof, wherein as compared with a wild type HPV66 L1 protein, the mutated HPV66 L1 protein has the following mutations:
(1) N-terminal truncation of 1-20 amino acids, for example, 1-20 amino acids, e.g. 1-5, 3-8, 5-10, 9-13, 10-15, 12-18 or 15-20 amino acids; and
(2) (a) substitution of amino acid residues at positions 265-283 of the wild type HPV66 L1 protein with amino acid residues at the corresponding positions of a L1 protein of a second type of wild-type HPV; or
and, the variant differs from the mutated HPV66 L1 protein only by substitution (preferably conservative substitution), addition or deletion of one or more (e.g. 1, 2, 3, 4, 5, 6, 7, 8, 9, 10 or 11) amino acids, and retains the function of the mutated HPV66 L1 protein, i.e. capability of inducing generation of neutralizing antibodies against at least two HPV types (e.g. HPV66 and HPV56, or HPV66, HPV56 and HPV53).
In some preferred embodiments, the mutated HPV66 L1 protein has the mutation as defined in (2) (b), and optionally, further has the following mutation:
(3) substitution of amino acid residues at positions 51-60 of the wild type HPV66 L1 protein with amino acid residues at the corresponding positions of a L1 protein of a third type of wild-type HPV, or
(4) substitution of amino acid residues at positions 114-150 of the wild type HPV66 L1 protein with amino acid residues at the corresponding positions of a L1 protein of a third type of wild-type HPV, or
(5) substitution of amino acid residues at positions 259-283 of the wild type HPV66 L1 protein with amino acid residues at the corresponding positions of a L1 protein of a third type of wild-type HPV.
In some preferred embodiments, the mutated HPV66 L1 protein has the mutations as defined in (2) (b) and (4), and optionally, further has the following mutation:
(6) substitution of amino acid residues at positions 172-181 of the wild type HPV66 L1 protein with amino acid residues at the corresponding positions of a L1 protein of a third type of wild-type HPV.
In some preferred embodiments, the mutated HPV66 L1 protein has 3, 5, 8, 10, 12, 15 or 18 amino acids truncated at N-terminal, as compared with the wild type HPV66 L1 protein.
In some preferred embodiments, the mutated HPV66 L1 protein has 5 amino acids truncated at N-terminal, as compared with the wild type HPV66 L1 protein.
In some preferred embodiments, the second type of wild-type HPV is HPV56. In some preferred embodiments, the amino acid residues at the corresponding positions as described in (2) (a) are amino acid residues at positions 265-283 of a wild type HPV56 L1 protein. In some preferred embodiments, the amino acid residues at the corresponding positions as described in (2) (b) are amino acid residues at positions 347-357 of a wild type HPV56 L1 protein.
In some preferred embodiments, the third type of wild-type HPV is HPV53. In some preferred embodiments, the amino acid residues at the corresponding positions as described in (3) are amino acid residues at positions 51-59 of a wild type HPV53 L1 protein. In some preferred embodiments, the amino acid residues at the corresponding positions as described in (4) are amino acid residues at positions 113-149 of a wild type HPV53 L1 protein. In some preferred embodiments, the amino acid residues at the corresponding positions as described in (5) are amino acid residues at positions 258-282 of a wild type HPV53 L1 protein. In some preferred embodiments, the amino acid residues at the corresponding positions as described in (6) are amino acid residues at positions 171-180 of a wild type HPV53 L1 protein.
In some preferred embodiments, the wild type HPV66 L1 protein has an amino acid sequence as set forth in SEQ ID NO: 1 or 28.
In some preferred embodiments, the wild type HPV56 L1 protein has an amino acid sequence as set forth in SEQ ID NO: 2.
In some preferred embodiments, the wild type HPV53 L1 protein has an amino acid sequence as set forth in SEQ ID NO: 3 or 31.
In some preferred embodiments, the amino acid residues at positions 347-357 of the wild type HPV56 L1 protein have a sequence as set forth in SEQ ID NO: 23.
In some preferred embodiments, the amino acid residues at positions 51-59 of the wild type HPV53 L1 protein have a sequence as set forth in SEQ ID NO: 24.
In some preferred embodiments, the amino acid residues at positions 113-149 of the wild type HPV53 L1 protein have a sequence as set forth in SEQ ID NO: 25.
In some preferred embodiments, the amino acid residues at positions 171-180 of the wild type HPV53 L1 protein have a sequence as set forth in SEQ ID NO: 65.
In some preferred embodiments, the amino acid residues at positions 258-282 of the wild type HPV53 L1 protein have a sequence as set forth in SEQ ID NO: 26.
In some preferred embodiments, the mutated HPV66 L1 protein has an amino acid sequence selected from the group consisting of: SEQ ID NO: 7, 8, 9, 10, 11 and 63.
In another aspect, the invention provides an isolated nucleic acid, encoding the mutated HPV66 L1 protein or a variant thereof as described above. In another aspect, the invention provides a vector comprising the isolated nucleic acid. In some preferred embodiments, the isolated nucleic acid according to the invention has a nucleotide sequence selected from the group consisting of: SEQ ID NO: 18, 19, 20, 21, 22 and 64.
Vectors useful for insertion of a polynucleotide of interest are well known in the art, including, but not limited to cloning vectors and expression vectors. In one embodiment, the vectors are, for example, plasmids, cosmids, phages, etc.
In another aspect, the invention further relates to a host cell comprising the isolated nucleic acid or the vector. The host cell includes, but is not limited to prokaryotic cells such as E. coli cells, and eukaryotic cells such as yeast cells, insect cells, plant cells and animal cells (such as mammalian cells, for example, mouse cells, human cells, etc.). The host cell according to the invention may also be a cell line, such as 293T cell.
In another aspect, the invention relates to a HPV virus-like particle, comprising or consisting of the mutated HPV66 L1 protein or a variant thereof according to the invention.
In some preferred embodiments, the HPV virus-like particle according to the invention comprises the mutated HPV66 L1 protein, which has N-terminal truncation of 1-20 amino acids, for example, 1-20 amino acids, e.g. 1-5, 3-8, 5-10, 9-13, 10-15, 12-18 or 15-20 amino acids, as compared to a wild type HPV66 L1 protein, and substitution of the amino acid residues at positions 347-357 of the wild type HPV66 L1 protein with the amino acid residues at positions 347-357 of a wild type HPV56 L1 protein.
In some preferred embodiments, the HPV virus-like particle according to the invention comprises the mutated HPV66 L1 protein, which has N-terminal truncation of 1-20 amino acids, for example, 1-20 amino acids, e.g. 1-5, 3-8, 5-10, 9-13, 10-15, 12-18 or 15-20 amino acids, as compared to a wild type HPV66 L1 protein, and substitution of the amino acid residues at positions 347-357 of the wild type HPV66 L1 protein with the amino acid residues at positions 347-357 of a wild type HPV56 L1 protein, and substitution of the amino acid residues at positions 51-60 of the wild type HPV66 L1 protein with the amino acid residues at positions 51-59 of a wild type HPV53 L1 protein.
In some preferred embodiments, the HPV virus-like particle according to the invention comprises the mutated HPV66 L1 protein, which has N-terminal truncation of 1-20 amino acids, for example, 1-20 amino acids, e.g. 1-5, 3-8, 5-10, 9-13, 10-15, 12-18 or 15-20 amino acids, as compared to a wild type HPV66 L1 protein, and substitution of the amino acid residues at positions 347-357 of the wild type HPV66 L1 protein with the amino acid residues at positions 347-357 of a wild type HPV56 L1 protein, and substitution of the amino acid residues at positions 114-150 of the wild type HPV66 L1 protein with the amino acid residues at positions 113-149 of a wild type HPV53 L1 protein.
In some preferred embodiments, the HPV virus-like particle according to the invention comprises the mutated HPV66 L1 protein, which has N-terminal truncation of 1-20 amino acids, for example, 1-20 amino acids, e.g. 1-5, 3-8, 5-10, 9-13, 10-15, 12-18 or 15-20 amino acids, as compared to a wild type HPV66 L1 protein, and substitution of the amino acid residues at positions 347-357 of the wild type HPV66 L1 protein with the amino acid residues at positions 347-357 of a wild type HPV56 L1 protein, and substitution of the amino acid residues at positions 259-283 of the wild type HPV66 L1 protein with the amino acid residues at positions 258-282 of a wild type HPV53 L1 protein.
In some preferred embodiments, the HPV virus-like particle according to the invention comprises the mutated HPV66 L1 protein, which has N-terminal truncation of 1-20 amino acids, for example, 1-20 amino acids, e.g. 1-5, 3-8, 5-10, 9-13, 10-15, 12-18 or 15-20 amino acids, as compared to a wild type HPV66 L1 protein, and substitution of the amino acid residues at positions 347-357 of the wild type HPV66 L1 protein with the amino acid residues at positions 347-357 of a wild type HPV56 L1 protein, and substitution of the amino acid residues at positions 114-150 of the wild type HPV66 L1 protein with the amino acid residues at positions 113-149 of a wild type HPV53 L1 protein, and substitution of the amino acid residues at positions 172-181 of the wild type HPV66 L1 protein with the amino acid residues at positions 171-180 of a wild type HPV53 L1 protein.
In a particularly preferred embodiment, the HPV virus-like particle according to the invention comprises the mutated HPV66 L1 protein, which has a sequence as set forth in SEQ ID NO: 7, 8, 9, 10, 11 or 63.
In another aspect, the invention further relates to a composition comprising the mutated HPV66 L1 protein or a variant thereof, the isolated nucleic acid, the vector, the host cell, or the HPV virus-like particle. In some preferred embodiments, the composition comprises the mutated HPV66 L1 protein or a variant thereof according to the invention. In some preferred embodiments, the composition comprises the HPV virus-like particle according to the invention.
In another aspect, the invention further relates to a pharmaceutical composition or vaccine, comprising the HPV virus-like particle according to the invention, and optionally a pharmaceutically acceptable carrier and/or excipient. The pharmaceutical composition or vaccine according to the invention can be used for preventing HPV infection, or a disease caused by HPV infection, such as cervical cancer and condyloma acuminatum.
In some preferred embodiments, the HPV virus-like particle is present in an amount effective for preventing HPV infection or a disease caused by HPV infection. In some preferred embodiments, the HPV infection is infection by one or more HPV types (e.g. HPV56 infection, HPV66 infection and/or HPV53 infection). In some preferred embodiments, the disease caused by HPV infection is selected from the group consisting of cervical cancer and condyloma acuminatum.
The pharmaceutical composition or vaccine according to the invention may be administrated by methods well known in the art, for example, but not limited to, orally or by injection. In the invention, a particularly preferred administration route is injection.
In some preferred embodiments, the pharmaceutical composition or vaccine according to the invention is administrated in a form of a unit dosage. For example, but not for limiting the invention, each unit dosage contains 5 μg-80 μg, preferably 20 μg-40 μg of HPV virus-like particle.
In another aspect, the invention relates to a method for preparing the mutated HPV66 L1 protein or a variant thereof as described above, comprising expressing the mutated HPV66 L1 protein or a variant thereof in a host cell, and then recovering the mutated HPV66 L1 protein or a variant thereof from a culture of the host cell.
In some preferred embodiments, the host cell is E. coli.
In some preferred embodiments, the method comprises the steps of: expressing the mutated HPV66 L1 protein or a variant thereof in E. coli, and then obtaining the mutated HPV66 L1 protein or a variant thereof by purifying a lysate supernatant of the E. coli. In some preferred embodiments, the mutated HPV66 L1 protein or a variant thereof is recovered from the lysate supernatant of the E. coli by chromatography (e.g. cation-exchange chromatography, hydroxyapatite chromatography and/or hydrophobic interaction chromatography).
In another aspect, the invention relates to a method for preparing a vaccine, comprising combining the HPV virus-like particle according to the invention with a pharmaceutically acceptable carrier and/or excipient.
In another aspect, the invention relates to a method for preventing HPV infection or a disease caused by HPV infection, comprising administering to a subject a prophylactically effective amount of the HPV virus-like particle or the pharmaceutical composition or vaccine according to the invention. In a preferred embodiment, the HPV infection is infection by one or more HPV types (e.g. HPV66 infection, HPV56 infection and/or HPV53 infection). In another preferred embodiment, the disease caused by HPV infection includes, but is not limited to cervical cancer and condyloma acuminatum. In another preferred embodiment, the subject is mammal, such as human.
In another aspect, the invention further relates to use of the mutated HPV66 L1 protein or a variant thereof or the HPV virus-like particle according to the invention in the manufacture of a pharmaceutical composition or vaccine for preventing HPV infection or a disease caused by HPV infection. In a preferred embodiment, the HPV infection is infection by one or more HPV types (e.g. HPV66 infection, HPV56 infection and/or HPV53 infection). In another preferred embodiment, the disease caused by HPV infection includes, but is not limited to, cervical cancer and condyloma acuminatum.
In another aspect, the invention further relates to the mutated HPV66 L1 protein or a variant thereof or the HPV virus-like particle according to the invention for the prevention of HPV infection or a disease caused by HPV infection. In a preferred embodiment, the HPV infection is infection by one or more HPV types (e.g. HPV66 infection, HPV56 infection and/or HPV53 infection). In another preferred embodiment, the disease caused by HPV infection includes, but is not limited to, cervical cancer and condyloma acuminatum.
In the invention, unless otherwise specified, the scientific and technical terms used herein have the meanings generally understood by a person skilled in the art. Moreover, the laboratory operations of cell culture, molecular genetics, nucleic acid chemistry, and immunology used herein are the routine operations widely used in the corresponding fields. Meanwhile, in order to better understand the invention, the definitions and explanations of the relevant terms are provided as follows.
According to the invention, the term “a second type of wild-type HPV” refers to a wild-type HPV type other than HPV66. In the invention, a second type of wild-type HPV is preferably wild type HPV56.
According to the invention, the term “a third type of wild-type HPV” refers to a wild-type HPV type other than HPV66 and the second type of wild-type HPV. In the invention, a third type of wild-type HPV is preferably wild type HPV53.
According to the invention, the expression “corresponding positions” refers to the equivalent positions of the sequences being compared when the sequences are optimally aligned, i.e. the sequences are aligned to obtain a highest percentage of identity.
According to the invention, the term “wild type HPV66 L1 protein” refers to the naturally-occurring major capsid protein L1 in Human Papillomavirus Type 66 (HPV66). The sequence of wild type HPV66 L1 protein is well known in the art, and can be found in public database (such as Accession No. ABO76865.1, Q80961.1, ABO76858.1 and ALT54961.1 in NCBI database).
In the invention, when an amino acid sequence of wild type HPV66 L1 protein is mentioned, it is described by reference to the sequence as set forth in SEQ ID NO: 1. For example, the expression “amino acid residues at positions 53-56 of a wild type HPV66 L1 protein” refers to the amino acid residues at positions 53-56 of the polypeptide as set forth in SEQ ID NO: 1. However, a person skilled in the art understands that wild type HPV66 may include various isolates, and there might be difference in the amino acid sequence of L1 protein among various isolates. Furthermore, a person skilled in the art understands that although there might be difference in sequence, the amino acid sequences of L1 protein have a very high identity (generally higher than 95%, e.g. higher than 96%, higher than 97%, higher than 98%, or higher than 99%) among different HPV66 isolates, and have substantively the same biological function. Therefore, in the invention, the term “wild type HPV66 L1 protein” includes not only the protein as set forth in SEQ ID NO: 1, but also L1 protein of various HPV66 isolates (such as HPV66 L1 protein as set forth in ABO76865.1, Q80961.1, ABO76858.1 and ALT54961.1). Moreover, when a sequence fragment of a wild type HPV66 L1 protein is described, it includes not only the sequence fragment of SEQ ID NO: 1, but also the corresponding sequence fragment of a L1 protein of various HPV66 isolates. For example, the expression “amino acid residues at positions 53-56 of a wild type HPV66 L1 protein” includes the amino acid residues at positions 53-56 of SEQ ID NO: 1, and the corresponding fragment of a L1 protein of various HPV66 isolates.
According to the invention, the term “wild type HPV56 L1 protein” refers to the naturally-occurring major capsid protein L1 in Human Papillomavirus Type 56 (HPV56). The sequence of wild type HPV56 L1 protein is well known in the art, and can be found in public database (such as Accession No. ALT54892.1, ALT54864.1, P36743.1 and ABO76830.1 in NCBI database).
In the invention, when an amino acid sequence of wild type HPV56 L1 protein is mentioned, it is described by reference to the sequence as set forth in SEQ ID NO: 2. For example, the expression “amino acid residues at positions 347-357 of a wild type HPV56 L1 protein” refers to the amino acid residues at positions 347-357 of the polypeptide as set forth in SEQ ID NO: 2. However, a person skilled in the art understands that wild type HPV56 may include various isolates, and there might be difference in the amino acid sequence of L1 protein among various isolates. Furthermore, a person skilled in the art understands that although there might be difference in sequence, the amino acid sequences of L1 protein have a very high identity (generally higher than 95%, e.g. higher than 96%, higher than 97%, higher than 98%, or higher than 99%) among different HPV56 isolates, and have substantively the same biological function. Therefore, in the invention, the term “wild type HPV56 L1 protein” includes not only the protein as set forth in SEQ ID NO: 2, but also L1 protein of various HPV56 isolates (such as HPV56 L1 protein as set forth in ALT54892.1, ALT54864.1, P36743.1 and ABO76830.1). Moreover, when a sequence fragment of a wild type HPV56 L1 protein is described, it includes not only the sequence fragment of SEQ ID NO: 2, but also the corresponding sequence fragment of a L1 protein of various HPV56 isolates. For example, the expression “amino acid residues at positions 347-357 of a wild type HPV56 L1 protein” includes the amino acid residues at positions 347-357 of SEQ ID NO: 2, and the corresponding fragment of a L1 protein of various HPV56 isolates.
According to the invention, the term “wild type HPV53 L1 protein” refers to the naturally-occurring major capsid protein L1 in Human Papillomavirus Type 53 (HPV53). The sequence of wild type HPV53 L1 protein is well known in the art, and can be found in public database (such as Accession No. NP041848.1, ANY26596.1, ABU54090.1 and ALJ32506.1 in NCBI database).
In the invention, when an amino acid sequence of wild type HPV53 L1 protein is mentioned, it is described by reference to the sequence as set forth in SEQ ID NO: 3. For example, the expression “amino acid residues at positions 51-59 of a wild type HPV53 L1 protein” refers to amino acid residues at positions 51-59 of the polypeptide as set forth in SEQ ID NO: 3. However, a person skilled in the art understands that wild type HPV53 may include various isolates, and there might be difference in the amino acid sequence of L1 protein among various isolates. Furthermore, a person skilled in the art understands that although there might be difference in sequence, the amino acid sequences of L1 protein have a very high identity (generally higher than 95%, e.g. higher than 96%, higher than 97%, higher than 98%, or higher than 99%) among different HPV53 isolates, and have substantively the same biological function. Therefore, in the invention, the term “wild type HPV53 L1 protein” includes not only the protein as set forth in SEQ ID NO: 3, but also L1 protein of various HPV53 isolates (such as HPV53 L1 protein as set forth in NP041848.1, ANY26596.1, ABU54090.1 and ALJ32506.1). Moreover, when a sequence fragment of a wild type HPV53 L1 protein is described, it includes not only the sequence fragment of SEQ ID NO: 3, but also the corresponding sequence fragment of L1 protein of various HPV53 isolates. For example, the expression “amino acid residues at positions 51-59 of a wild type HPV53 L1 protein” includes the amino acid residues at positions 51-59 of SEQ ID NO: 3, and the corresponding fragment of L1 protein of various HPV53 isolates.
According to the invention, the expression “corresponding sequence fragments” or “corresponding fragments” refers to the fragments that are located at equivalent positions of the sequences being compared when the sequences are optimally aligned, i.e. the sequences are aligned to obtain a highest percentage of identity.
According to the invention, the expression “N-terminal truncation of X amino acids” or “having X amino acids truncated at N-terminal” refers to substitution of the amino acid residues from positions 1 to X at the N-terminal of a protein with methionine residue encoded by an initiator codon (for initiating protein translation). For example, a HPV66 L1 protein having 5 amino acids truncated at N-terminal refers to a protein resulted from substituting the amino acid residues from positions 1 to 5 at the N-terminal of wild type HPV66 L1 protein with methionine residue encoded by an initiator codon.
According to the invention, the term “variant” refers to a protein, whose amino acid sequence has substitution (preferably conservative substitution), addition or deletion of one or more (e.g. 1, 2, 3, 4, 5, 6, 7, 8 or 9) amino acids, or has an identity of at least 90%, 95%, 96%, 97%, 98%, or 99%, as compared with the mutated HPV66 L1 protein according to the invention (for example, the protein as set forth in SEQ ID NO: 7, 8, 9, 10 or 11), and which retains a function of the mutated HPV66 L1 protein according to the invention. In the invention, the term “function of the mutated HPV66 L1 protein” refers to a capability of inducing generation of neutralizing antibodies against at least two HPV types (e.g. HPV66 and HPV56, or HPV66, HPV56 and HPV53). The term “identity” refers to a measure of similarity between nucleotide sequences or amino acid sequences. Generally, sequences were aligned to obtain a maximum matching. “Identity” has well-known meanings in the art and can be calculated by published algorithm (such as BLAST).
According to the invention, the term “identity” refers to the match degree between two polypeptides or between two nucleic acids. When two sequences for comparison have the same monomer sub-unit of base or amino acid at a certain site (e.g., each of two DNA molecules has an adenine at a certain site, or each of two polypeptides has a lysine at a certain site), the two molecules are identical at the site. The percent identity between two sequences is a function of the number of identical sites shared by the two sequences over the total number of sites for comparison×100. For example, if 6 of 10 sites of two sequences are matched, these two sequences have an identity of 60%. For example, DNA sequences: CTGACT and CAGGTT share an identity of 50% (3 of 6 sites are matched). Generally, the comparison of two sequences is conducted in a manner to produce maximum identity. Such alignment can be conducted by for example using a computer program such as Align program (DNAstar, Inc.) which is based on the method of Needleman, et al. (J. Mol. Biol. 48:443-453, 1970). The percent identity between two amino acid sequences can also be determined using the algorithm of E. Meyers and W. Miller (Comput. Appl. Biosci., 4:11-17 (1988)) which has been incorporated into the ALIGN program (version 2.0), using a PAM120 weight residue table, and with a gap length penalty of 12 and a gap penalty of 4. In addition, the percentage of identity between two amino acid sequences can be determined by the algorithm of Needleman and Wunsch (J. Mol. Biol. 48:444-453 (1970)) which has been incorporated into the GAP program in the GCG software package (available at http://www.gcg.com), using either a Blossum 62 matrix or a PAM250 matrix, and with a gap weight of 16, 14, 12, 10, 8, 6, or 4 and a length weight of 1, 2, 3, 4, 5, or 6.
As used herein, the term “conservative substitution” refers to amino acid substitutions which would not disadvantageously affect or change the essential properties of a protein/polypeptide comprising the amino acid sequence. For example, a conservative substitution may be introduced by standard techniques known in the art such as site-directed mutagenesis and PCR-mediated mutagenesis. Conservative amino acid substitutions include substitutions wherein an amino acid residue is substituted with another amino acid residue having a similar side chain, for example, a residue physically or functionally similar (such as, having similar size, shape, charge, chemical property including the capability of forming covalent bond or hydrogen bond, etc.) to the corresponding amino acid residue. The families of amino acid residues having similar side chains have been defined in the art. These families include amino acids having basic side chains (for example, lysine, arginine and histidine), amino acids having acidic side chains (for example, aspartic acid and glutamic acid), amino acids having uncharged polar side chains (for example, glycine, asparagine, glutamine, serine, threonine, tyrosine, cysteine, and tryptophan), amino acids having nonpolar side chains (for example, alanine, valine, leucine, isoleucine, proline, phenylalanine, and methionine), amino acids having β-branched side chains (such as threonine, valine, and isoleucine) and amino acids having aromatic side chains (for example, tyrosine, phenylalanine, tryptophan, and histidine). Therefore, generally a conservative substitution refers to a substitution of a corresponding amino acid residue with another amino acid residue from the same side-chain family. Methods for identifying amino acid conservative substitutions are well known in the art (see, for example, Brummell et al., Biochem. 32: 1180-1187 (1993); Kobayashi et al., Protein Eng. 12(10): 879-884 (1999); and Burks et al., Proc. Natl. Acad. Sci. USA 94: 412-417 (1997), which are incorporated herein by reference).
According to the invention, the term “E. coli expression system” refers to an expression system consisting of E. coli (strain) and a vector, wherein the E. coli (strain) is derived from the commercially available strains, including, but not limited to: ER2566, BL21 (DE3), B834 (DE3), and BLR (DE3).
According to the invention, the term “vector” refers to a nucleic acid carrier tool which can have a polynucleotide inserted therein. When the vector allows for the expression of the protein encoded by the polynucleotide inserted therein, the vector is called an expression vector. The vector can have the carried genetic material elements expressed in a host cell by transformation, transduction, or transfection into the host cell. Vectors are well known by a person skilled in the art, including, but not limited to plasmids, phages, cosmids, etc.
According to the invention, the term “a pharmaceutically acceptable carrier and/or excipient” refers to a carrier and/or excipient that is pharmacologically and/or physiologically compatible to a subject and active ingredients, which is well known in the art (see, for example, Remington's Pharmaceutical Sciences. Edited by Gennaro A R, 19th ed. Pennsylvania: Mack Publishing Company, 1995), including, but not limited to: pH regulators, surfactants, adjuvants, and ionic strength enhancers. For example, pH regulators include, but are not limited to, phosphate buffers; surfactants include, but are not limited to: cation surfactants, anion surfactants, or non-ionic surfactants, e.g., Tween-80; adjuvants include, but are not limited to, aluminium adjuvant (e.g., aluminium hydroxide), and Freund's adjuvant (e.g., Freund's complete adjuvant); and ionic strength enhancers include, but are not limited to, NaCl.
According to the invention, the term “an effective amount” refers to an amount that can effectively achieve the intended purpose. For example, an amount effective for preventing a disease (such as HPV infection) refers to an amount effective for preventing, suppressing, or delaying the occurrence of a disease (such as HPV infection). The determination of such an effective amount is within the ability of a person skilled in the art.
According to the invention, the term “chromatography” includes, but is not limited to: ion exchange chromatography (such as cation-exchange chromatography), hydrophobic interaction chromatography, absorbent chromatography (such as hydroxyapatite chromatography), gel filtration chromatography (gel exclusion chromatography), and affinity chromatography.
According to the invention, the term “lysate supernatant” refers to a solution produced by the following steps: host cells (such as E. coli) are disrupted in a lysis buffer, and the insoluble substances are then removed from the lysed solution containing the disrupted host cells. Various lysis buffers are well known in the art, including, but not limited to Tris buffers, phosphate buffers, HEPES buffers, MOPS buffers, etc. In addition, the disrupting of a host cell can be accomplished by methods well known by a person skilled in the art, including, but not limited to homogenizer disrupting, ultrasonic treatment, grinding, high pressure extrusion, lysozyme treatment, etc. Methods for removing insoluble substances are also well known by a person skilled in the art, including, but not limited to filtration and centrifugation.
Studies show that although there is certain cross-protection between HPV66 and other HPV type(s) (such as HPV56 and HPV53), such cross-protection is very low, generally lower than one percent, even one thousandth of the protection level of VLP of the same HPV type. Therefore, a subject vaccinated with HPV66 vaccine, still has a high risk of being infected by other HPV type(s) (such as HPV56 and HPV53).
The invention provides a mutated HPV66 L1 protein and a HPV virus-like particle formed by the same. The HPV virus-like particle according to the invention can provide significant cross-protection against HPV66 and other HPV type(s) (such as HPV56 and HPV53). Especially, at the same immunizing dose, the HPV virus-like particle according to the invention can induce the generation of high-titer neutralizing antibodies against at least two HPV types (e.g. HPV66 and HPV56, or HPV66, HPV56 and HPV53) in organisms, and its effect is comparable to that of a mixture of VLPs of multiple HPV types (e.g. a mixture of HPV66 VLP and HPV56 VLP, or a mixture of HPV66 VLP, HPV56 VLP and HPV53 VLP). Therefore, the HPV virus-like particle according to the invention can be used to prevent infection by at least two HPV types (e.g. HPV66 and HPV56, or HPV66, HPV56 and HPV53) at the same time as well as diseases associated with the infection, and has significantly beneficial technical effects. This has particularly significant advantages in terms of extending the protection range of HPV vaccines and reducing the production cost of HPV vaccines.
The embodiments of the invention are further described in detail by reference to the drawings and examples. However, a person skilled in the art would understand that the following drawings and examples are intended for illustrating the invention only, rather than defining the scope of the invention. According to the detailed description of the following drawings and preferred embodiments, various purposes and advantages of the invention are apparent for a person skilled in the art.
Some of the sequences involved in the invention are provided in the following Table 1.
The present invention is further described by reference to the examples as follows, wherein the examples are used only for the purpose of illustrating the present invention, rather than limiting the present invention.
Unless indicated otherwise, the molecular biological experimental methods and immunological assays used in the present invention are carried out substantially in accordance with the methods as described in J. Sambrook et al., Molecular Cloning: A Laboratory Manual (Second Edition), Cold Spring Harbor Laboratory Press, 1989, and F. M. Ausubel et al., Short Protocols in Molecular Biology, 3rd Edition, John Wiley & Sons, Inc., 1995; and restriction enzymes are used under the conditions recommended by the manufacturers. Those skilled in the art understand that the examples are used for illustrating the present invention, but not intended to limit the protection scope of the present invention.
Construction of Expression Vectors
An expression vector encoding the mutated HPV66 L1 protein comprising a segment from HPV56 L1 protein was constructed by PCR for multi-site mutagenesis, wherein the initial template used was the plasmid pTO-T7-HPV66N5C (encoding the HPV66 L1 protein having 5 amino acids truncated at N-terminal; abbreviated as 66L1N5 in Table 2). The templates and primers for each PCR were shown in Table 2, and the amplification conditions for PCR were as followed: denaturation at 94° C. for 2 min; 30 cycles (denaturation at 98° C. for 10 sec, annealing at a given temperature for a certain period of time, and extension at 58° C. for 6.5 min); and final extension at 68° C. for 10 min. The temperature and time of annealing were listed in Table 2. The sequences of the PCR primers used were listed in Table 3.
To the amplification product (50 μL), 2 μL restriction endonuclease DpnI (Fermentas (MBI), Cat. No. FD1704, 2500U/tube) was added, and the resultant mixture was incubated at 37° C. for 60 min. 10 μL of the product of digestion was used to transform 40 μL competent E. coli ER2566 (purchased from New England Biolabs) prepared by the Calcium chloride method. The transformed E. coli was spread onto solid LB medium (the components of the LB medium: 10 g/L peptone, 5 g/L yeast powder, 10 g/L NaCl, the same hereinafter) containing kanamycin (at a final concentration of 25 μg/mL, the same hereinafter), and was subjected to static culture at 37° C. for 10-12 h until single colonies could be observed clearly. Single colony was picked and inoculated into a tube containing 4 mL liquid LB medium (containing kanamycin), and cultured with shaking at 220 rpm for 10 h at 37° C., and then 1 ml bacterial solution was taken and stored at −70° C. Plasmids were extracted from E. coli, and T7 primer was used to sequence the nucleotide sequences of the fragments of interest inserted into the plasmids. The sequencing result showed that the nucleotide sequences of the fragments of interest inserted into the constructed plasmids (expression vectors) were SEQ ID NO: 15 and 17, respectively, and their encoded amino acid sequences were SEQ ID NO: 4 and 6, respectively (the corresponding proteins were designated as H66N5-56T1 and H66N5-56T3, respectively).
The mutated protein H66N5-56T1 differs from HPV66N5 by: the substitution of the amino acid residues from positions 53-56 of wild type HPV66 L1 protein with the amino acid residues from positions 53-56 of wild type HPV56 L1 protein. The mutated protein H66N5-56T3 differs from HPV66N5 by: the substitution of the amino acid residues from positions 178-180 of wild type HPV66 L1 protein with the amino acid residues from positions 178-180 of wild type HPV56 L1 protein.
Gibson assembly (Gibson D G, Young L, Chuang R Y, Venter J C, Hutchison C A, Smith H O. Enzymatic assembly of DNA molecules up to several hundred kilobases. Nat Methods. 2009; 6:343-5. doi: 10.1038/nmeth.1318) was used to construct the expression vector encoding the other mutated HPV66 L1 protein, wherein the mutated HPV66 L1 protein comprised a specific segment from HPV56 L1 and a specific segment from HPV53L1. In brief, a short fragment comprising mutations and a long fragment comprising no mutation were obtained by PCR, and Gibson assembly system was then used to ligate the two fragments to form a ring. The initial template used comprised the plasmid pTO-T7-HPV66L1N5 (encoding the HPV66 L1 protein having 5 amino acids truncated at N-terminal; abbreviated as 66L1N5 in Table 2), the plasmid pTO-T7-HPV53N0 (encoding the full-length HPV56 L1 protein; abbreviated as 56L1N0 in Table 2), the plasmid pTO-T7-H66N5-56T5 (encoding the mutated protein H66N5-56T5; abbreviated as H66N5-56T5 in Table 2) and the plasmid pTO-T7-HPV53N5 (encoding the HPV53 L1 protein having 5 amino acids truncated at N-terminal; abbreviated as 53L1N5 in Table 2). The templates and primers for each PCR were shown in Table 2, and, the amplification conditions for PCR for amplifying the short fragment were as followed: denaturation at 94° C. for 10 min; 25 cycles (denaturation at 94° C. for 50 sec, annealing at a given temperature for a certain period of time, and extension at 72° C. for 1 min); and final extension at 72° C. for 10 min. The amplification conditions for PCR for amplifying the long fragment were as followed: denaturation at 94° C. for 10 min; 25 cycles (denaturation at 94° C. for 50 sec, annealing at a given temperature for a certain period of time, and extension at 72° C. for 7.5 min); and final extension at 72° C. for 10 min. The sequences of the PCR primers used were listed in Table 3. The amplification product was subjected to electrophoresis, the fragment of interest was then recovered by using DNA Extraction Kit (BEYOTIME, Cat. No. D0033), and its concentration was determined. The short fragment and long fragment obtained by amplification were mixed at a molar ratio of 2:1 (a total volume of 3 μL), and 3 μL of 2×Gibson Assembly Master Mix (purchased from NEB, containing T5 exonuclease, Phusion DNA polymerase, Taq DNA ligase) was then added, and reacted at 50° C. for 1 h.
The assembled product (6 μL) was used to transform 40 μL competent E. coli ER2566 (purchased from New England Biolabs) prepared by the Calcium chloride method. The transformed E. coli were spread onto solid LB medium containing kanamycin, and were subjected to static culture at 37° C. for 10-12 h until single colonies could be observed clearly. Single colony was picked and inoculated into a tube containing 4 mL liquid LB medium (containing kanamycin), and cultured with shaking at 220 rpm for 10h at 37° C., and then 1 ml bacterial solution was taken and stored at −70° C. Plasmids were extracted from E. coli, and T7 primer was used to sequence the nucleotide sequences of the fragments of interest inserted into the plasmids. The sequencing result showed that the nucleotide sequences of the fragments of interest inserted into the constructed plasmids (expression vectors) were SEQ ID NO: 16, 18, 19, 20, 21 and 22, respectively, and their encoded amino acid sequences were SEQ ID NO: 5, 7, 8, 9, 10 and 11, respectively (the corresponding proteins were designated as H66N5-56T2, H66N5-56T4, H66N5-56T5, H66N5-56T5-53S1, H66N5-56T5- 53S2 and H66N5-56T5-53S4, respectively).
The H66N5-56T5-53S2-53S3 gene was synthesized by Sangon Biotech (Shanghai) Co., Ltd. The synthesized plasmid comprising the HPV66N5-56T5-53S2-53S3 gene was digested with NdeI and SalI (at 37° C. for 12h). After digestion, the gene of interest was recovered by using DNA Extraction Kit (BEYOTIME, Cat. No. D0033), and the digested H66N5-56T5-53S2-53S3 gene was ligated with pTO-T7 vector at 16° C. for 12 h, and then the resultant product was used to transform competent E. coli ER2566 (purchased from New England Biolabs). The transformed E. coli were spread onto solid LB medium containing kanamycin, and were subjected to static culture at 37° C. for 10-12 h until single colonies could be observed clearly. Single colony was picked and inoculated into a tube containing 4 mL liquid LB medium (containing kanamycin), and cultured with shaking at 220 rpm for 10h at 37° C., and then 1 ml bacterial solution was taken and stored at −70° C. Plasmids were extracted from E. coli, and T7 primer was used to sequence the nucleotide sequences of the fragments of interest inserted into the plasmids. The sequencing result showed that the nucleotide sequences of the fragments of interest inserted into the constructed plasmids (expression vectors) was SEQ ID NO: 64, and its encoded amino acid sequences were SEQ ID NO: 63 (the corresponding proteins were designated as H66N5-56T5-53S2-53S3).
The mutated protein H66N5-56T2 differs from HPV66N5 by: the substitution of the amino acid residues from positions 130-150 of wild type HPV66 L1 protein with the amino acid residues from positions 130-150 of wild type HPV56 L1 protein. The mutated protein H66N5-56T4 differs from HPV66N5 by: the substitution of the amino acid residues from positions 265-283 of wild type HPV66 L1 protein with the amino acid residues from positions 265-283 of wild type HPV56 L1 protein. The mutated protein H66N5-56T5 differs from HPV66N5 by: the substitution of the amino acid residues from positions 347-357 of wild type HPV66 L1 protein with the amino acid residues from positions 347-357 of wild type HPV56 L1 protein.
The mutated protein H66N5-56T5-53S1 differs from HPV66N5 by: the substitution of the amino acid residues from positions 347-357 of wild type HPV66 L1 protein with the amino acid residues from positions 347-357 of wild type HPV56 L1 protein, and the substitution of the amino acid residues from positions 51-60 of wild type HPV66 L1 protein with the amino acid residues from positions 51-59 of wild type HPV53 L1 protein. The mutated protein H66N5-56T5-53S2 differs from HPV66N5 by: the substitution of the amino acid residues from positions 347-357 of wild type HPV66 L1 protein with the amino acid residues from positions 347-357 of wild type HPV56 L1 protein, and the substitution of the amino acid residues from positions 114-150 of wild type HPV66 L1 protein with the amino acid residues from positions 113-149 of wild type HPV53 L1 protein. The mutated protein H66N5-56T5-53S4 differs from HPV66N5 by: the substitution of the amino acid residues from positions 347-357 of wild type HPV66 L1 protein with the amino acid residues from positions 347-357 of wild type HPV56 L1 protein, and the substitution of the amino acid residues from positions 259-283 of wild type HPV66 L1 protein with the amino acid residues from positions 258-282 of wild type HPV53 L1 protein.
The mutated protein H66N5-56T5-53S2-53S3 differs from HPV66N5 by: the substitution of the amino acid residues from positions 347-357 of wild type HPV66 L1 protein with the amino acid residues from positions 347-357 of wild type HPV56 L1 protein, and the substitution of the amino acid residues from positions 114-150 of wild type HPV66 L1 protein with the amino acid residues from positions 113-149 of wild type HPV53 L1 protein, and the substitution of the amino acid residues from positions 172-181 of wild type HPV66 L1 protein with the amino acid residues from positions 171-180 of wild type HPV53 L1 protein.
Expression of the Mutated Proteins on a Large Scale
The E. coli solutions comprising the recombinant plasmid pTO-T7-H66N5-56T1, pTO-T7-H66N5-56T2, pTO-T7-H66N5-56T3, pTO-T7-H66N5-56T4, pTO-T7-H66N5-56T5, pTO-T7-H66N5-56T5-53S1, pTO-T7-H66N5-56T5-53S2, pTO-T7-H66N5-56T5-53S4 and pTO-T7-H66N5-56T5-53S2-53S3, respectively, were taken from −70° C. refrigerator, were inoculated in 100 mL LB liquid medium containing kanamycin, and incubated at 200 rpm and 37° C. for about 8 h. Then, the culture was transferred to 500 mL LB medium containing kanamycin (1 ml bacterial solution was transferred), and was further incubated. When the bacterial concentration reached an OD600 of about 0.6, the culturing temperature was lowered to 25° C. and 500 μL IPTG was added to each culture bottle. The incubation was further performed for 8 h. After the incubation was finished, the bacteria were collected by centrifugation. The bacteria expressing H66N5-56T1, H66N5-56T2, H66N5-56T3, H66N5-56T4, H66N5-56T5, H66N5-56T5-53S1, H66N5-56T5-53S2, H66N5-56T5-53S4 and H66N5-56T5-53S2-53S3 protein were obtained, respectively.
Disruption of Bacteria Expressing the Mutated Proteins
The bacteria obtained were re-suspended at a ratio of 1 g bacteria to 10 mL lysis buffer (20 mM Tris buffer, pH7.2, 300 mM NaCl). The bacteria were disrupted by using an ultrasonic apparatus for 30 min. The lysis solution containing the disrupted bacteria were centrifuged at 13500 rpm (30000 g) for 15 min, and the supernatant (i.e. the supernatant of disrupted bacteria) was obtained.
Chromatographic Purification of the Mutated Protein
Equipment: AKTA Explorer 100 preparative liquid chromatography system produced by GE Healthcare (i.e. the original Amershan Pharmacia Co.)
Chromatographic media: SP Sepharose 4 Fast Flow (GE Healthcare Co.), CHT-II (purchased from Bio-RAD) and Butyl Sepharose 4 Fast Flow (GE Healthcare Co.)
Buffer: Buffer A (20 mM phosphate buffer, pH8.0, 20 mM DTT); and Buffer B (20 mM phosphate buffer, pH8.0, 20 mM DTT, 2M NaCl). The buffers containing different concentrations of NaCl used in the following elution protocol were prepared by mixing Buffer A and Buffer B at a certain ratio.
Sample: the supernatants of disrupted bacteria containing H66N5-56T1, H66N5-56T2, H66N5-56T3, H66N5-56T4, H66N5-56T5, H66N5-56T5-53S1, H66N5-56T5-53S2, H66N5- 56T5-53S4 and H66N5-56T5-53S2-53S3, respectively, as obtained above.
Elution Protocol:
(1) Cation exchange purification of the supernatant of disrupted bacteria by SP Sepharose 4 Fast Flow: the sample was loaded on the column, undesired proteins were then eluted with a buffer containing 400 mM NaCl (80% Buffer A+20% Buffer B), followed by the elution of the protein of interest with a buffer containing 800 mM NaCl (60% Buffer A+40% Buffer B), and the fraction eluted with the buffer containing 800 mM NaCl was collected;
(2) Chromatographic purification of the elution fraction obtained in the step (1) by CHTII (hydroxyapatite chromatography): the elution fraction obtained in the step (1) was diluted so that the NaCl concentration was decreased to 0.5 M; the sample was loaded on the column, undesired proteins were then eluted with a buffer containing 500 mM NaCl (75% Buffer A+25% Buffer B), followed by the elution of the protein of interest with a buffer containing 1000 mM NaCl (50% Buffer A+50% Buffer B), and the fraction eluted with the buffer containing 1000 mM NaCl was collected;
(3) Chromatographic purification of the elution fraction obtained in the step (2) by HIC (hydrophobic interaction chromatography): the sample was loaded on the column, undesired proteins were then eluted with a buffer containing 1000 mM NaCl, followed by the elution of the protein of interest with a buffer containing 200 mM NaCl (90% Buffer A+10% Buffer B), and the fraction eluted with the buffer containing 200 mM NaCl was collected.
150 μL of elution fraction obtained in the step (3) was added to 30 μL of 6× Loading Buffer (1 L of which contained 300 ml of 1M TB 6.8, 600 ml of 100% glycerol, 120 g of SDS, 6 g of bromophenol blue, and 50 ml of β-mercaptoethanol). The resultant solution was mixed well and incubated in 80° C. water bath for 10 min. 10 μl of the resultant sample was then subjected to 10% SDS-PAGE at 120V for 120 min; and the electrophoretic bands were stained by Coomassie brilliant blue. The electrophoretic result was shown in
By similar methods, HPV66N5 protein was prepared and purified by using E. coli and the plasmid pTO-T7-HPV66N5; HPV56N0 protein was prepared and purified by using E. coli and the plasmid pTO-T7-HPV56L1N0; and HPV53N5 protein was prepared and purified by using E. coli and the plasmid pTO-T7-HPV53N5.
Western Blot Assay of the Mutated Proteins
The H66N5-56T1, H66N5-56T2, H66N5-56T3, H66N5-56T4, H66N5-56T5, H66N5-56T5-53S1, H66N5-56T5-53S2 and H66N5-56T5-53S4 protein purified by the method above were subjected to electrophoresis. After electrophoresis, Western Blot assay was carried out by using a broad-spectrum antibody 4B3 against HPV L1 protein, and the result was shown in
A given volume (about 2 ml) of the protein H66N5-56T1, H66N5-56T2, H66N5-56T3, H66N5-56T4, H66N5-56T5, H66N5-56T5-53S1, H66N5-56T5-53S2, H66N5-56T5-53S4 or H66N5-56T5-53S2-53S3, was dialyzed to (1) 2 L storage buffer (20 mM sodium phosphate buffer pH 6.5, 0.5 M NaCl); (2) 2 L renaturation buffer (50 mM sodium phosphate buffer pH 6.0, 2 mM CaCl2, 2 mM MgCl2, 0.5 M NaCl); and (3) 20 mM sodium phosphate buffer pH 7.0, 0.5 M NaCl, successively. The dialysis was performed in each of the three buffers for 12 h.
By similar methods, the HPV66N5, HPV56N0 and HPV53N5 protein were assembled into HPV66N5 VLP, HPV56N0 VLP and HPV53N5 VLP, respectively.
Molecular Sieve Chromatographic Analysis
The dialyzed sample was subjected to molecular sieve chromatographic analysis by 1120 Compact LC High Performance Liquid Chromatographic System (Agilent Technologies), wherein the analytical column used was TSK Gel PW5000×1 7.8×300 mm. The analysis results were shown in
Sedimentation Velocity Analysis
The apparatus for sedimentation velocity analysis was Beckman XL-A Analytical Ultracentrifuge, equipped with optical inspection system and An-50Ti and An-60Ti rotor. The sedimentation coefficients of H66N5-56T1 VLP, H66N5-56T2 VLP, H66N5-56T3 VLP, H66N5-56T4 VLP, H66N5-56T5 VLP, H66N5-56T5-53S1 VLP, H66N5-56T5-53S2 VLP, H66N5-56T5-53S4 VLP, H66N5-56T5-53S2-53S3 VLPHPV56N0 VLP, HPV66N5 VLP and HPV53N5 VLP were analyzed by sedimentation velocity method. The results were shown in
Morphological Test of Virus-Like Particles
A 100 μL sample comprising VLP was observed by transmission electron microscope (TEM). The apparatus used was a 100 kV Transmission Electron Microscope supplied by JEOL Ltd. (100,000× magnification). In brief, a 13.5 μL sample was negatively stained with 2% phosphotungstic acid (pH 7.0), fixed on a carbon-coated copper grid, and then observed by TEM. The results were shown in
In this experiment, virus-like particles used were H66N5-56T1 VLP, H66N5-56T2 VLP, H66N5-56T3 VLP, H66N5-56T4 VLP and H66N5-56T5 VLP.
In this experiment, vaccination schedule was shown in Table 4. All the mice (6-week old BalB/c female mice) were divided into 3 groups: Aluminum adjuvant group 1 (at an immunizing dose of 5 μg, using aluminum adjuvant), Aluminum adjuvant group 2 (at an immunizing dose of 1 μg, using aluminum adjuvant), and Aluminum adjuvant group 3 (at an immunizing dose of 0.2 μg, using aluminum adjuvant). Each group was further divided into 8 subgroups. The Control subgroups 1 and 2 were vaccinated with HPV66N5 VLP alone and HPV56N0 VLP alone, respectively, the Control subgroup 3 was vaccinated with the mixed HPV66/HPV56 VLP (i.e. a mixture of HPV66N5 VLP and HPV56N0 VLP, at a given immunizing dose for each VLP). The Experimental subgroups 1, 2, 3, 4 and 5 were vaccinated with H66N5-56T1VLP, H66N5-56T2VLP, H66N5-56T3VLP, H66N5-56T4VLP and H66N5-56T5 VLP, respectively.
In Aluminum adjuvant groups 1-3, 5 mice/subgroup were vaccinated by intraperitoneal injection, at an immunizing dose of 5 μg, 1 μg, and 0.2 μg, respectively, and an injection volume of 1 mL. All the mice were subjected to the first vaccination at Week 0, and then subjected to the booster vaccination at Weeks 2 and 4, respectively. At Week 6, blood sample was collected via orbital bleeding, and the titers of antibodies against HPV66 and HPV56 in serum were analyzed. The analysis results were shown in
In this experiment, virus-like particles used were H66N5-56T4 VLP and H66N5-56T5 VLP. 6-Week old BalB/c female mice (8 mice) were vaccinated with aluminum adjuvant by single intraperitoneal injection, wherein H66N5-56T4 VLP or H66N5-56T5 VLP was used in the Experimental groups, and HPV56N0 VLP alone, HPV66N5 VLP alone or the mixed HPV66/HPV56 VLP (i.e. a mixture of HPV66N5 VLP and HPV56N0 VLP) was used in the Control groups; the immunizing dose was 0.900 μg, 0.300 μg, 0.100 μg, 0.033 μg or 0.011 μg; the immunizing volume was 1 mL. In addition, the diluent used to dilute the vaccine was used as a blank control. 8 Mice were vaccinated in each group, and at Week 5 after vaccination, venous blood was collected from eyeball. Antibodies against HPV in the serum were detected, and by Reed-Muench method (Reed L J M H. A simple method of estimating fifty percent endpoints. Am J Hyg. 1938; 27:493-7), ED50 for inducing seroconversion (i.e. inducing the generation of antibodies in mice) was calculated for each sample. The results were shown in Tables 5-9.
96%
The results showed that 5 weeks after vaccination of mice, ED50 of H66N5-56T5 VLP for inducing the generation of antibodies against HPV66 in mice was comparable to that of HPV66N5 VLP alone, and was significantly superior to that of HPV56N0 VLP alone; and its ED50 of for inducing the generation of antibodies against HPV56 in mice was slightly weaker than that of HPV56N0 VLP alone, but was significantly superior to that of HPV66N5 VLP alone. This showed that H66N5-56T5 VLP had good cross-immunogenicity and cross-protection against HPV66 and HPV56.
In this experiment, virus-like particles used were H66N5-56T5-53S1 VLP, H66N5-56T5-53S2 VLP and H66N5-56T5-53S4 VLP.
In this experiment, vaccination schedule was shown in Table 10. All the mice (6-week old BalB/c female mice) were divided into 2 groups: Aluminum adjuvant group 1 (at an immunizing dose of 5 μg, using aluminum adjuvant), and Aluminum adjuvant group 2 (at an immunizing dose of 1 μg, using aluminum adjuvant). Each group was further divided into 7 subgroups. The Control subgroups 1, 2 and 3 were vaccinated with HPV66N5 VLP alone, HPV56N0 VLP alone and HPV53N5 VLP alone, respectively, the Control subgroup 4 was vaccinated with the mixed HPV66/56/53 VLP (i.e. a mixture of HPV66N5 VLP, HPV56N0 VLP and HPV53N5 VLP, at a given immunizing dose for each VLP). The Experimental subgroups 1, 2 and 3 were vaccinated with H66N5-56T5-53S1 VLP, H66N5-56T5-53S2 VLP and H66N5-56T5-53S4 VLP, respectively.
In Aluminum adjuvant groups 1-2, 5 mice/subgroup were vaccinated by intraperitoneal injection, at an immunizing dose of 5 μg and 1 μg, respectively, and an injection volume of 1 mL. All the mice were subjected to the first vaccination at Week 0, and then subjected to the booster vaccination at Weeks 2 and 4, respectively. At Week 6, blood sample was collected via orbital bleeding, and the titers of antibodies against HPV66, HPV56 and HPV53 in serum were analyzed. The analysis results were shown in
In this experiment, the virus-like particle used was H66N5-56T5-53S2-53S3 VLP.
In this experiment, vaccination schedule was shown in Table 11. All the mice (6-week old BalB/c female mice) were divided into 2 groups: Experimental group (at an immunizing dose of 5 μg, using aluminum adjuvant), and Control group (at an immunizing dose of 5 μg, using aluminum adjuvant). Each Control group was further divided into 4 subgroups. The Control subgroups 1, 2 and 3 were vaccinated with HPV66N5 VLP alone, HPV56N0 VLP alone and HPV53N5 VLP alone, respectively; the Control subgroup 4 was vaccinated with the mixed HPV66/56/53 VLP (i.e. a mixture of HPV66N5 VLP, HPV56N0 VLP and HPV53N5 VLP, at a given immunizing dose for each VLP). The Experimental subgroup was vaccinated with H66N5-56T5-53S2-53S3 VLP.
5 Mice/subgroup were vaccinated by intraperitoneal injection, at an immunizing dose of 5 μg, and an injection volume of 1 mL. All the mice were subjected to the first vaccination at Week 0, and then subjected to the booster vaccination at Weeks 2 and 4, respectively. At Week 6, blood sample was collected via orbital bleeding, and the titers of antibodies against HPV66, HPV56 and HPV53 in serum were analyzed. The analysis results were shown in
Although the specific embodiments of the present invention have been described in details, those skilled in the art would understand that, according to the teachings disclosed in the specification, various modifications and changes can be made thereto, and that such modifications and changes are within the scope of the present invention. The scope of the present invention is given by the appended claims and any equivalents thereof.
Number | Date | Country | Kind |
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201810563504.2 | Jun 2018 | CN | national |
Filing Document | Filing Date | Country | Kind |
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PCT/CN2019/089940 | 6/4/2019 | WO |
Publishing Document | Publishing Date | Country | Kind |
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WO2019/233400 | 12/12/2019 | WO | A |
Number | Name | Date | Kind |
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6551597 | Harrison | Apr 2003 | B1 |
Number | Date | Country |
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101914139 | Nov 2021 | CN |
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