Modified M2 proteins produce heterotypic immunity against influenza A virus
Identifieur interne : 001990 ( Main/Exploration ); précédent : 001989; suivant : 001991Modified M2 proteins produce heterotypic immunity against influenza A virus
Auteurs : A. Michael Frace [États-Unis] ; Alexander I. Klimov [États-Unis] ; Thomas Rowe [États-Unis] ; Renee A. Black [États-Unis] ; Jacqueline M. Katz [États-Unis]Source :
- Vaccine [ 0264-410X ] ; 1999.
English descriptors
- Teeft :
- Amino acid sequence, Antibody epitope, Antibody response, Antigenic, Arlington heights, Cell culture, Cell density, Coding region, Control groups, Deletion, Deletion proteins, Elsevier science, Epitope, Escherichia coli, Extracellular domain, Frace, Full length, Fusion protein, Fusion proteins, General virology, Glutathione sepharose, Heterologous, Heterotypic immunity, Highest dilution, Immunogenic properties, Individual sera, Induction period, Insect cells, Intracellular domain, Lung virus titers, Lytic properties, Major neutralizing antigen, Mice vaccinated, Mouse, Overnight cultures, Ovine cysticercosis, Pasteur merieux connaught, Primer, Prokaryotic expression, Protein, Recombinant, Recombinant products, Serum antibody, Ssm2, Standard deviations, Surface expression, Synthetic peptide, Titer, Transmembrane, Transmembrane domain, Vaccinated, Vaccination, Vaccine, Viral, Viral clearance, Virology, Virus, Virus replication, Virus titer reductions, Western blot, Whole virus vaccine.
Abstract
Abstract: Vaccination with the influenza A transmembrane protein M2 provides enhanced viral clearance and recovery from influenza A virus infection in mice. However, the high degree of hydrophobicity of the protein limits its purification for vaccine purposes. We have attempted to alter the structure of the M2 protein to allow high level recombinant expression in Escherichia coli, to reduce its hydrophobicity and improve protein solubility, thus improving its properties as a vaccine subunit candidate. Constructs investigated include deletion of the transmembrane domain of M2 (residues 26–43) and an extended deletion (residues 26–55). A full-length M2 protein was not pursued because of poor expression, even in the presence of amantadine. Expressed as glutathione S-transferase fusion proteins and used to vaccinate mice, either deletion construct was found to raise M2-specific serum antibodies and enhance viral clearance in mice challenged with homologous and heterologous influenza A viruses. Enzymatic cleavage from the GST fusion domain produces soluble protein giving similar results. The results demonstrate that large alterations of M2 protein structure can improve its isolation and purification characteristics without detracting from its immunogenic properties.
Url:
DOI: 10.1016/S0264-410X(99)00005-5
Affiliations:
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Katz</name><affiliation wicri:level="2"><country xml:lang="fr">États-Unis</country><wicri:regionArea>Influenza Branch, Division of Viral and Rickettsial Diseases, National Center for Infectious Diseases, Centers for Disease Control and Prevention, 1600 Clifton Road, Atlanta, GA 30333</wicri:regionArea><placeName><region type="state">Géorgie (États-Unis)</region></placeName></affiliation></author></analytic><monogr></monogr><series><title level="j">Vaccine</title><title level="j" type="abbrev">JVAC</title><idno type="ISSN">0264-410X</idno><imprint><publisher>ELSEVIER</publisher><date type="published" when="1999">1999</date><biblScope unit="volume">17</biblScope><biblScope unit="issue">18</biblScope><biblScope unit="page" from="2237">2237</biblScope><biblScope unit="page" to="2244">2244</biblScope></imprint><idno type="ISSN">0264-410X</idno></series></biblStruct></sourceDesc><seriesStmt><idno type="ISSN">0264-410X</idno></seriesStmt></fileDesc><profileDesc><textClass><keywords scheme="Teeft" xml:lang="en"><term>Amino acid sequence</term><term>Antibody epitope</term><term>Antibody response</term><term>Antigenic</term><term>Arlington heights</term><term>Cell culture</term><term>Cell density</term><term>Coding region</term><term>Control groups</term><term>Deletion</term><term>Deletion proteins</term><term>Elsevier science</term><term>Epitope</term><term>Escherichia coli</term><term>Extracellular domain</term><term>Frace</term><term>Full length</term><term>Fusion protein</term><term>Fusion proteins</term><term>General virology</term><term>Glutathione sepharose</term><term>Heterologous</term><term>Heterotypic immunity</term><term>Highest dilution</term><term>Immunogenic properties</term><term>Individual sera</term><term>Induction period</term><term>Insect cells</term><term>Intracellular domain</term><term>Lung virus titers</term><term>Lytic properties</term><term>Major neutralizing antigen</term><term>Mice vaccinated</term><term>Mouse</term><term>Overnight cultures</term><term>Ovine cysticercosis</term><term>Pasteur merieux connaught</term><term>Primer</term><term>Prokaryotic expression</term><term>Protein</term><term>Recombinant</term><term>Recombinant products</term><term>Serum antibody</term><term>Ssm2</term><term>Standard deviations</term><term>Surface expression</term><term>Synthetic peptide</term><term>Titer</term><term>Transmembrane</term><term>Transmembrane domain</term><term>Vaccinated</term><term>Vaccination</term><term>Vaccine</term><term>Viral</term><term>Viral clearance</term><term>Virology</term><term>Virus</term><term>Virus replication</term><term>Virus titer reductions</term><term>Western blot</term><term>Whole virus vaccine</term></keywords></textClass><langUsage><language ident="en">en</language></langUsage></profileDesc></teiHeader><front><div type="abstract" xml:lang="en">Abstract: Vaccination with the influenza A transmembrane protein M2 provides enhanced viral clearance and recovery from influenza A virus infection in mice. However, the high degree of hydrophobicity of the protein limits its purification for vaccine purposes. We have attempted to alter the structure of the M2 protein to allow high level recombinant expression in Escherichia coli, to reduce its hydrophobicity and improve protein solubility, thus improving its properties as a vaccine subunit candidate. Constructs investigated include deletion of the transmembrane domain of M2 (residues 26–43) and an extended deletion (residues 26–55). A full-length M2 protein was not pursued because of poor expression, even in the presence of amantadine. Expressed as glutathione S-transferase fusion proteins and used to vaccinate mice, either deletion construct was found to raise M2-specific serum antibodies and enhance viral clearance in mice challenged with homologous and heterologous influenza A viruses. Enzymatic cleavage from the GST fusion domain produces soluble protein giving similar results. The results demonstrate that large alterations of M2 protein structure can improve its isolation and purification characteristics without detracting from its immunogenic properties.</div></front></TEI><affiliations><list><country><li>États-Unis</li></country><region><li>Géorgie (États-Unis)</li><li>Pennsylvanie</li></region></list><tree><country name="États-Unis"><region name="Pennsylvanie"><name sortKey="Frace, A Michael" sort="Frace, A Michael" uniqKey="Frace A" first="A. Michael" last="Frace">A. Michael Frace</name></region><name sortKey="Black, Renee A" sort="Black, Renee A" uniqKey="Black R" first="Renee A" last="Black">Renee A. Black</name><name sortKey="Katz, Jacqueline M" sort="Katz, Jacqueline M" uniqKey="Katz J" first="Jacqueline M" last="Katz">Jacqueline M. Katz</name><name sortKey="Klimov, Alexander I" sort="Klimov, Alexander I" uniqKey="Klimov A" first="Alexander I" last="Klimov">Alexander I. Klimov</name><name sortKey="Rowe, Thomas" sort="Rowe, Thomas" uniqKey="Rowe T" first="Thomas" last="Rowe">Thomas Rowe</name></country></tree></affiliations></record>Pour manipuler ce document sous Unix (Dilib)
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