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Open AccessJournal ArticleDOI

Polymerase chain reaction amplification and typing of rotavirus nucleic acid from stool specimens.

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TLDR
A PCR typing method was devised in which each human serotype virus produced a characteristic segment size, readily identifiable in agarose gels, which provided a rapid and efficient means of obtaining large quantities of cDNA suitable for sequencing, cloning, and other genetic studies, precluding the need for cell culture and virus purification.
Abstract
The rotavirus gene segment coding for the major outer capsid glycoprotein vp7 was amplified directly from stool specimens by the polymerase chain reaction (PCR). Double-stranded RNA extracted from stool samples was used as the template for reverse transcription, which was followed immediately and in the same reaction mix with amplification, using the Taq polymerase. Various conditions were examined to optimize the yield of the amplified gene. The concentrations of MgCl2, dimethyl sulfoxide, and template RNA were critical. The choice of primer pairs allowed amplification of the entire segment or specific portions. By using type-specific primers derived from distinct regions on the gene, we devised a PCR typing method in which each human serotype virus produced a characteristic segment size, readily identifiable in agarose gels. The PCR typing method was applied to 10 rotavirus reference strains, including all 6 known human serotypes (serotypes 1, 2, 3, 4, 8, and 9), and to 34 stool specimens previously serotyped by an enzyme immunoassay with monoclonal antibodies. An absolute correlation was found between the molecular and serologic methods. In addition, 14 stool specimens nonserotypable by an enzyme immunoassay with monoclonal antibodies could be typed by the PCR method. Besides the application for rotavirus detection and typing directly from stools, the PCR method provides a rapid and efficient means of obtaining large quantities of cDNA suitable for sequencing, cloning, and other genetic studies, precluding the need for cell culture and virus purification.

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Journal ArticleDOI

Expanding global distribution of rotavirus serotype G9: detection in Libya, Kenya, and Cuba.

TL;DR: Serotype G9 may be the fifth most common human rotavirus serotype, after serotypes G1 to G4, and future humanRotavirus vaccines will need to protect against disease caused by this serotype.
Journal ArticleDOI

Mixed viral infections causing acute gastroenteritis in children in a waterborne outbreak.

TL;DR: To conclude, massive exposure to several AGE viruses caused mixed infections and severe AGE regardless of the aetiological agents.
Journal ArticleDOI

Rotavirus Strains Bearing Genotype G9 or P[9] Recovered from Brazilian Children with Diarrhea from 1997 to 1999

TL;DR: Human rotavirus strains belonging to genotype G9 or P[9] were detected in a collection of stool specimens from children with diarrhea in two cities of the state of Rio de Janeiro, Brazil, between March 1997 and December 1999, suggesting a genetic similarity between the Brazilian G3:P[ 9] strains and the Japanese virus, which is similar to a feline rotav virus genetically.
Journal ArticleDOI

Epidemiology of Acute Viral Gastroenteritis in Children Hospitalized in Rouen, France

TL;DR: The epidemiologic characteristics of acute viral gastroenteritis in hospitalized children, including the more-frequent dehydration observed among children with rotavirus versus those with astrovirus or calicivirus gastroEnteritis, were assessed and enteral rehydration was more rapidly achieved in patients with gastroenterococci.
References
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Book ChapterDOI

Specific synthesis of DNA in vitro via a polymerase-catalyzed chain reaction.

TL;DR: A method whereby a nucleic acid sequence can be exponentially amplified in vitro is described in the chapter, and the possibility of utilizing a heat-stable DNA polymerase is explored so as to avoid the need for addition of new enzyme after each cycle of thermal denaturation.
Journal ArticleDOI

Diagnosis of chronic myeloid and acute lymphocytic leukemias by detection of leukemia-specific mRNA sequences amplified in vitro.

TL;DR: D diagnosis of chronic myeloid and acute lymphocytic leukemias by this procedure is rapid, much more sensitive than existing protocols, and independent of the presence or absence of an identifiable Philadelphia chromosome.
Journal Article

Polymerase chain reaction

Oste C
- 01 Feb 1988 - 
Journal ArticleDOI

Serotypic Similarity and Diversity of Rotaviruses of Mammalian and Avian Origin as Studied by Plaque-Reduction Neutralization

TL;DR: A surprising observation that emerged from this study was the existence of a rotavirus (porcine strain SB-1A) bridging serotypes 4 and 5, which was identified in both humans and pigs.
Journal ArticleDOI

Production and preliminary characterization of monoclonal antibodies directed at two surface proteins of rhesus rotavirus.

TL;DR: Thirty-six monoclonal antibodies immunoprecipitated the 82-kilodalton outer capsid protein, the product of the fourth gene, the viral hemagglutinin, and neutralized rhesus rotavirus to moderate or high titer.
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