Rapid detection of influenza A neuraminidase subtypes by cDNA amplification coupled to a simple DNA enzyme immunoassay
Identifieur interne : 001E22 ( Main/Exploration ); précédent : 001E21; suivant : 001E23Rapid detection of influenza A neuraminidase subtypes by cDNA amplification coupled to a simple DNA enzyme immunoassay
Auteurs : B. Schweiger [Allemagne] ; I. Lange [Allemagne] ; R. Heckler [Allemagne] ; H. Willers [Allemagne] ; E. Schreier [Allemagne]Source :
- Archives of Virology [ 0304-8608 ] ; 1994-09-01.
Descripteurs français
- KwdFr :
- ADN complémentaire (analyse), ADN complémentaire (génétique), Données de séquences moléculaires, Génome viral, Hybridation d'acides nucléiques, Réaction de polymérisation en chaîne, Sensibilité et spécificité, Sialidase (), Sialidase (génétique), Sondes d'ADN, Séquence nucléotidique, Techniques immunoenzymatiques, Virus de la grippe A (), Virus de la grippe A (enzymologie), Virus de la grippe A (génétique).
- MESH :
- analyse : ADN complémentaire.
- enzymologie : Virus de la grippe A.
- génétique : ADN complémentaire, Sialidase, Virus de la grippe A.
- Pascal (Inist)
- Anticorps monoclonal, Données de séquences moléculaires, Détection, Exo-α-sialidase, Génome viral, Hybridation d'acides nucléiques, Hybridation moléculaire, Influenzavirus A, Méthode, Méthode immunoenzymatique, Réaction chaîne polymérase, Réaction de polymérisation en chaîne, Sensibilité et spécificité, Sialidase, Sondes d'ADN, Spécificité type, Séquence nucléotidique, Technique ELISA, Techniques immunoenzymatiques, Virus de la grippe A.
English descriptors
- KwdEn :
- Base Sequence, DNA Probes, DNA, Complementary (analysis), DNA, Complementary (genetics), Detection, ELISA assay, Enzyme immunoassay, Exo-α-sialidase, Genome, Viral, Immunoenzyme Techniques, Influenza A virus (classification), Influenza A virus (enzymology), Influenza A virus (genetics), Influenzavirus A, Method, Molecular Sequence Data, Molecular hybridization, Monoclonal antibody, Neuraminidase (classification), Neuraminidase (genetics), Nucleic Acid Hybridization, Polymerase Chain Reaction, Polymerase chain reaction, Sensitivity and Specificity, Type specificity.
- MESH :
- chemical , analysis : DNA, Complementary.
- chemical , classification : Neuraminidase.
- chemical , genetics : DNA, Complementary, Neuraminidase.
- chemical : DNA Probes.
- classification : Influenza A virus.
- enzymology : Influenza A virus.
- genetics : Influenza A virus.
- Base Sequence, Genome, Viral, Immunoenzyme Techniques, Molecular Sequence Data, Nucleic Acid Hybridization, Polymerase Chain Reaction, Sensitivity and Specificity.
- Teeft :
- Amplification, Arch virol, Assay, Cdna, Cdna amplification, Chemiluminescent detection, Complete nucleotide sequence, Deia, Embryonated eggs, Enzyme immunoassay, Ethidium bromide, Federal republic, Human influenza, Human influenza virus, Hybridization, Hybridization procedures, Immunoassay, Influenza, Influenza virus, Influenza virus neuraminidase gene, Influenza viruses, Large number, Microtiter, Microtiter wells, Neuraminidase, Neuraminidase gene, Neuraminidase subtypes, Optical density, Polymerase, Polymerase chain reaction, Primer, Rapid detection, Rapid diagnosis, Respiratory secretions, Schreier, Schweiger, Specific probe, Subtypes, Subtyping, Uninfected allantoic fluid, Universal primers, Virol, Virol methods, Virology, Virus strains.
Abstract
Summary: A newly developed colorimetric method, DNA enzyme immunoassay (DEIA), was applied to the detection of neuraminidase subtypes N1 and N2 of influenza A viruses. Reverse transcription and polymerase chain reaction with universal primers were used for genomic amplification of H1N1, H2N2, and H3N2 strains. Following amplification, an aliquot of the PCR product was hybridized to biotinylated DNA sequences (N1/N2 probes) immobilized on microtiter wells. The hybridization event was revealed by monoclonal antibodies to double stranded DNA in a standard ELISA reaction. The assay described here was able to distinguish accurately between the two neuraminidase subtypes of human influenza A viruses. It is a simple and rapid method facilitating the handling of a large number of samples and therefore seems to be easily applicable to diagnostic laboratories.
Url:
DOI: 10.1007/BF01310805
Affiliations:
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Le document en format XML
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strains</term></keywords></textClass><langUsage><language ident="en">en</language></langUsage></profileDesc></teiHeader><front><div type="abstract" xml:lang="en">Summary: A newly developed colorimetric method, DNA enzyme immunoassay (DEIA), was applied to the detection of neuraminidase subtypes N1 and N2 of influenza A viruses. Reverse transcription and polymerase chain reaction with universal primers were used for genomic amplification of H1N1, H2N2, and H3N2 strains. Following amplification, an aliquot of the PCR product was hybridized to biotinylated DNA sequences (N1/N2 probes) immobilized on microtiter wells. The hybridization event was revealed by monoclonal antibodies to double stranded DNA in a standard ELISA reaction. The assay described here was able to distinguish accurately between the two neuraminidase subtypes of human influenza A viruses. It is a simple and rapid method facilitating the handling of a large number of samples and therefore seems to be easily applicable to diagnostic laboratories.</div></front></TEI><affiliations><list><country><li>Allemagne</li></country><region><li>Basse-Saxe</li><li>Berlin</li></region><settlement><li>Berlin</li><li>Hanovre</li></settlement></list><tree><country name="Allemagne"><region name="Berlin"><name sortKey="Schweiger, B" sort="Schweiger, B" uniqKey="Schweiger B" first="B." last="Schweiger">B. Schweiger</name></region><name sortKey="Heckler, R" sort="Heckler, R" uniqKey="Heckler R" first="R." last="Heckler">R. Heckler</name><name sortKey="Lange, I" sort="Lange, I" uniqKey="Lange I" first="I." last="Lange">I. Lange</name><name sortKey="Schreier, E" sort="Schreier, E" uniqKey="Schreier E" first="E." last="Schreier">E. Schreier</name><name sortKey="Willers, H" sort="Willers, H" uniqKey="Willers H" first="H." last="Willers">H. 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