A procedure for the isolation of specific point mutants of influenza virus
Identifieur interne : 004664 ( Main/Merge ); précédent : 004663; suivant : 004665A procedure for the isolation of specific point mutants of influenza virus
Auteurs : Bradley M. Mitchell ; Dan C. DebordeSource :
- Journal of Virological Methods [ 0166-0934 ] ; 1993.
English descriptors
- Teeft :
- Allantoic fluid, Amplification, Congenic influenza virus, Consensus sequence, Deborde, Dextran sulfate, Embryonated, Embryonated chicken eggs, Embryonated eggs, Embryonated eggs inoculated, Enami, Equal volume, Gene sequence, Growth advantage, Hybridization, Individual eggs, Infectious virions, Infectious virus, Influenza, Influenza virus, Influenza viruses, Inoculum, Maassab, Major sequence, Mdck, Mdck cells, Mutant, Mutant virus, Mutation, Nitrocellulose paper, Oligodeoxynucleotide, Oligodeoxynucleotide probe, Palese, Particular probe, Phenotypic significance, Plaque, Point mutation, Polynucleotide kinase, Positive hybridization signal, Positive signal, Prehybridization buffer, Primer extension, Probe, Probe panel, Rare point, Rare sequence, Rare transfectant, Relative abundance, Room temperature, Screen vrna, Screening step, Selective conditions, Selective pressure, Sequencing, Several rounds, Single base, Sodium acetate, Specific point mutants, Temperature sensitivity, Tissue culture cells, Viral, Virion, Virus, Virus sample, Vrna.
Abstract
Abstract: Procedures were developed for the screening and isolation of RNA viruses that vary from the consensus population by a single point mutation and are present in low abundance. We tested these procedures using a mixture of the vaccine donor line cold-adapted (ca) B/Ann Arbor/1/66 and its wild type (wt) progenitor at a ratio of 1,000:1. A 13-mer oligodeoxynucleotide was prepared as a [32P]-radiolabeled probe which specifically hybridized to wt viral RNA (vRNA) at a region that varied between the ca and wt sequence by a single base at position 1,320 of the PA gene. This probe was able to detect as little as 88 pg of total wt vRNA blotted to nitrocellulose, while giving no positive signal with as much as 1 μg of total ca vRNA. We were able to isolate virus containing the wt PA gene sequence from the mixed pool of ca and wt viruses by two successive rounds of amplification in embryonated eggs inoculated with a controlled number of infectious virions. During each round of amplification the abundance of the virus containing the wt PA gene sequence was increased about ten-fold. Once a relative abundance of 1:10 was reached, the virus was cloned by plaquing in Madin-Darby canine kidney cells. These procedures, which allow the isolation of specific point mutants, utilize no selective pressure conditions and are suitable for analyzing the phenotypic importance of known mutations in biologically important viruses.
Url:
DOI: 10.1016/0166-0934(93)90031-L
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<record><TEI wicri:istexFullTextTei="biblStruct"><teiHeader><fileDesc><titleStmt><title>A procedure for the isolation of specific point mutants of influenza virus</title><author><name sortKey="Mitchell, Bradley M" sort="Mitchell, Bradley M" uniqKey="Mitchell B" first="Bradley M." last="Mitchell">Bradley M. Mitchell</name></author><author><name sortKey="Deborde, Dan C" sort="Deborde, Dan C" uniqKey="Deborde D" first="Dan C." last="Deborde">Dan C. Deborde</name></author></titleStmt><publicationStmt><idno type="wicri:source">ISTEX</idno><idno type="RBID">ISTEX:23AF5E6ED1B730CEAE73718BA765DA331125E0B6</idno><date when="1993" year="1993">1993</date><idno type="doi">10.1016/0166-0934(93)90031-L</idno><idno type="url">https://api.istex.fr/ark:/67375/6H6-KLP9P48M-J/fulltext.pdf</idno><idno type="wicri:Area/Istex/Corpus">001582</idno><idno type="wicri:explorRef" wicri:stream="Istex" wicri:step="Corpus" wicri:corpus="ISTEX">001582</idno><idno type="wicri:Area/Istex/Curation">001582</idno><idno type="wicri:Area/Istex/Checkpoint">001C09</idno><idno type="wicri:explorRef" wicri:stream="Istex" wicri:step="Checkpoint">001C09</idno><idno type="wicri:doubleKey">0166-0934:1993:Mitchell B:a:procedure:for</idno><idno type="wicri:Area/Main/Merge">004664</idno></publicationStmt><sourceDesc><biblStruct><analytic><title level="a">A procedure for the isolation of specific point mutants of influenza virus</title><author><name sortKey="Mitchell, Bradley M" sort="Mitchell, Bradley M" uniqKey="Mitchell B" first="Bradley M." last="Mitchell">Bradley M. Mitchell</name><affiliation><wicri:noCountry code="subField">MTUSA</wicri:noCountry></affiliation></author><author><name sortKey="Deborde, Dan C" sort="Deborde, Dan C" uniqKey="Deborde D" first="Dan C." last="Deborde">Dan C. Deborde</name><affiliation><wicri:noCountry code="subField">MTUSA</wicri:noCountry></affiliation></author></analytic><monogr></monogr><series><title level="j">Journal of Virological Methods</title><title level="j" type="abbrev">VIRMET</title><idno type="ISSN">0166-0934</idno><imprint><publisher>ELSEVIER</publisher><date type="published" when="1993">1993</date><biblScope unit="volume">42</biblScope><biblScope unit="issue">2–3</biblScope><biblScope unit="page" from="181">181</biblScope><biblScope unit="page" to="191">191</biblScope></imprint><idno type="ISSN">0166-0934</idno></series></biblStruct></sourceDesc><seriesStmt><idno type="ISSN">0166-0934</idno></seriesStmt></fileDesc><profileDesc><textClass><keywords scheme="Teeft" xml:lang="en"><term>Allantoic fluid</term><term>Amplification</term><term>Congenic influenza virus</term><term>Consensus sequence</term><term>Deborde</term><term>Dextran sulfate</term><term>Embryonated</term><term>Embryonated chicken eggs</term><term>Embryonated eggs</term><term>Embryonated eggs inoculated</term><term>Enami</term><term>Equal volume</term><term>Gene sequence</term><term>Growth advantage</term><term>Hybridization</term><term>Individual eggs</term><term>Infectious virions</term><term>Infectious virus</term><term>Influenza</term><term>Influenza virus</term><term>Influenza viruses</term><term>Inoculum</term><term>Maassab</term><term>Major sequence</term><term>Mdck</term><term>Mdck cells</term><term>Mutant</term><term>Mutant virus</term><term>Mutation</term><term>Nitrocellulose paper</term><term>Oligodeoxynucleotide</term><term>Oligodeoxynucleotide probe</term><term>Palese</term><term>Particular probe</term><term>Phenotypic significance</term><term>Plaque</term><term>Point mutation</term><term>Polynucleotide kinase</term><term>Positive hybridization signal</term><term>Positive signal</term><term>Prehybridization buffer</term><term>Primer extension</term><term>Probe</term><term>Probe panel</term><term>Rare point</term><term>Rare sequence</term><term>Rare transfectant</term><term>Relative abundance</term><term>Room temperature</term><term>Screen vrna</term><term>Screening step</term><term>Selective conditions</term><term>Selective pressure</term><term>Sequencing</term><term>Several rounds</term><term>Single base</term><term>Sodium acetate</term><term>Specific point mutants</term><term>Temperature sensitivity</term><term>Tissue culture cells</term><term>Viral</term><term>Virion</term><term>Virus</term><term>Virus sample</term><term>Vrna</term></keywords></textClass><langUsage><language ident="en">en</language></langUsage></profileDesc></teiHeader><front><div type="abstract" xml:lang="en">Abstract: Procedures were developed for the screening and isolation of RNA viruses that vary from the consensus population by a single point mutation and are present in low abundance. We tested these procedures using a mixture of the vaccine donor line cold-adapted (ca) B/Ann Arbor/1/66 and its wild type (wt) progenitor at a ratio of 1,000:1. A 13-mer oligodeoxynucleotide was prepared as a [32P]-radiolabeled probe which specifically hybridized to wt viral RNA (vRNA) at a region that varied between the ca and wt sequence by a single base at position 1,320 of the PA gene. This probe was able to detect as little as 88 pg of total wt vRNA blotted to nitrocellulose, while giving no positive signal with as much as 1 μg of total ca vRNA. We were able to isolate virus containing the wt PA gene sequence from the mixed pool of ca and wt viruses by two successive rounds of amplification in embryonated eggs inoculated with a controlled number of infectious virions. During each round of amplification the abundance of the virus containing the wt PA gene sequence was increased about ten-fold. Once a relative abundance of 1:10 was reached, the virus was cloned by plaquing in Madin-Darby canine kidney cells. These procedures, which allow the isolation of specific point mutants, utilize no selective pressure conditions and are suitable for analyzing the phenotypic importance of known mutations in biologically important viruses.</div></front></TEI></record>Pour manipuler ce document sous Unix (Dilib)
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