Detection of hepatitis A virus, rotavirus, and enterovirus in naturally contaminated shellfish and sediment by reverse transcription-seminested PCR

Detection of hepatitis A virus, rotavirus, and enterovirus in naturally contaminated shellfish and sediment by reverse transcription-seminested PCR

A reverse transcription-PCR method was developed to detect enterovirus (EV), hepatitis A virus (HAV), and rotavirus (RV) RNAs in shellfish and sediment. The method was first tested under experimental conditions by using virus-spiked shellfish to evaluate assay sensitivity. The use of CC41 cellulose...

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Veröffentlicht in:Applied and Environmental Microbiology 1994-10, Vol.60 (10), p.3665-3671
Hauptverfasser: Le Guyader, F, Dubois, E, Menard, D, Pommepuy, M
Format: Artikel
Sprache:eng
Schlagworte:
ALMEJAS
AMPLIFICATION CHAINE POLYMERASE
Animals
ATLANTICO NORDESTE
ATLANTIQUE NORD EST
Base Sequence
BIOCHIMIE
BIODEGRADACION
BIODEGRADATION
Biology
BIOQUIMICA
BIVALVIA
CLAM
CRASSOSTREA GIGAS
DNA Probes - genetics
DNA, Viral - genetics
ENTEROVIRUS
Enterovirus - genetics
Enterovirus - isolation & purification
Food contamination & poisoning
Food Microbiology
FRANCE
FRANCIA
Hepatitis
hepatitis A virus
Hepatovirus - genetics
Hepatovirus - isolation & purification
HUITRE
Humans
INFECCION
INFECTION
Marine
MEJILLON
METHODE
METODOS
Molecular Sequence Data
MOULE
MYTILUS EDULIS
OSTRA
Polymerase Chain Reaction - methods
Polymerase Chain Reaction - statistics & numerical data
REACCION DE CADENAS DE POLIMERASA
Ribonucleic acid
RNA
RNA, Viral - genetics
RNA, Viral - isolation & purification
ROTAVIRUS
Rotavirus - genetics
Rotavirus - isolation & purification
SEDIMENT
SEDIMENTO
Sensitivity and Specificity
Shellfish
Shellfish - microbiology
Soils
Viruses
Water Microbiology
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Beschreibung
Zusammenfassung:A reverse transcription-PCR method was developed to detect enterovirus (EV), hepatitis A virus (HAV), and rotavirus (RV) RNAs in shellfish and sediment. The method was first tested under experimental conditions by using virus-spiked shellfish to evaluate assay sensitivity. The use of CC41 cellulose was found to be efficient for removing inhibitors of RV detection. For sediment samples, a Sephadex column was used to allow the detection of EV and HAV RNAs. The specificity of amplified products was controlled by hybridization with digoxigenin-labeled oligoprobes. The method was then applied to naturally contaminated shellfish and sediments. EV, HAV, and RV RNAs were detected in 22, 14, and 20% of the shellfish samples, respectively. No relationship between viral contamination and bacterial contamination was found. When viral RNAs (HAV or EV) were detected in sediments, they were also detected in shellfish
ISSN:0099-2240
1098-5336
DOI:10.1128/aem.60.10.3665-3671.1994