Detection of adenoviruses in stools from healthy persons and patients with diarrhea by two‐step polymerase chain reaction
Identifieur interne : 004835 ( Main/Exploration ); précédent : 004834; suivant : 004836Detection of adenoviruses in stools from healthy persons and patients with diarrhea by two‐step polymerase chain reaction
Auteurs : Annika Allard [Suède] ; Bo Albinsson [Suède] ; Göran Wadell [Suède]Source :
- Journal of Medical Virology [ 0146-6615 ] ; 1992-06.
English descriptors
- Teeft :
- Acute stage, Adenovirus, Adenovirus infections, Adenovirus particles, Adenovirus type, Adenovirus types, Agarose, Allard, American journal, Amplification, Amplification system, Amplimer, Diarrheal disease, Different adenovirus types, Different sets, Eads, England biolabs, Enteric, Enteric adenovirus, Enteric adenoviruses, Final concentration, General hexon primers, Healthy adults, Healthy children, Hexon, Hexon primers, Human adenoviruses, Hybridization, Molecular weight standards, Monoclonal antibodies, Negative controls, Orion diagnostica, Polymerase, Polymerase chain reaction, Primer, Primer pair, Reaction mixture, Restriction enzyme analysis, Second amplification, Serotypes, Specific primers, Stool, Stool sample, Stool samples, Stool specimens, Subgenus, Toogood, Unpublished data, Viral, Virology, Virus particles, Wadell, Young children.
Abstract
The use of the polymerase chain reaction (PCR) for detection of human adenoviruses in diluted stool samples was investigated. Two sets of nested primers, including primers specific for the hexon‐coding region and for the E1 B region of enteric adenoviruses (EAd), were assessed by two‐step amplification. The primers constitute two different PCR systems designed for the detection of adenoviruses belonging to all six subgenera (A‐F), and the two EAds Ad40 and Ad41, respectively. In a two‐step PCR mediated amplification a single virus particle was detected when the two sets of general hexon primers or Ead specific primers were used. Earlier results from PCR detection of adenoviruses in stool from children suffering from diarrhea gave indications that adenovirus particles are commonly shed in stools without being identified as the cause of il I ness [Allard et a I.: Journal of Clinical Microbiology 28:2659‐2667, 1990]). Therefore, the general and the EAd specific PCR assays were assessed on 150 stool specimens from three groups including 50 healthy children, 50 healthy adults, and 50 adults suffering from diarrhea. When the two sets of general hexon primers were used, 25 of the 50 specimens from the healthy children (mean age 21 months) were found positive by two‐step PCR amplification. Nine of the 50 specimens from the healthy adults (mean age 32 years) were found positive whereas 12 of the 50 specimens from sick adults (mean age 31 years) gave amplification products, using the two sets of general hexon primers in a nested fashion. None of the 150 specimens were found to be positive by two‐step PCR amplification using the two sets of EAd‐specific primers. The sensitivity of the PCR, together with its simplicity and reduced time scale compared to other detection methods, support the potential of this technique as an additional method for routine detection of human adenovirus infections. © 1992 Wiley‐Liss, Inc.
Url:
DOI: 10.1002/jmv.1890370214
Affiliations:
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infections</term><term>Adenovirus particles</term><term>Adenovirus type</term><term>Adenovirus types</term><term>Agarose</term><term>Allard</term><term>American journal</term><term>Amplification</term><term>Amplification system</term><term>Amplimer</term><term>Diarrheal disease</term><term>Different adenovirus types</term><term>Different sets</term><term>Eads</term><term>England biolabs</term><term>Enteric</term><term>Enteric adenovirus</term><term>Enteric adenoviruses</term><term>Final concentration</term><term>General hexon primers</term><term>Healthy adults</term><term>Healthy children</term><term>Hexon</term><term>Hexon primers</term><term>Human adenoviruses</term><term>Hybridization</term><term>Molecular weight standards</term><term>Monoclonal antibodies</term><term>Negative controls</term><term>Orion diagnostica</term><term>Polymerase</term><term>Polymerase chain reaction</term><term>Primer</term><term>Primer pair</term><term>Reaction mixture</term><term>Restriction enzyme analysis</term><term>Second amplification</term><term>Serotypes</term><term>Specific primers</term><term>Stool</term><term>Stool sample</term><term>Stool samples</term><term>Stool specimens</term><term>Subgenus</term><term>Toogood</term><term>Unpublished data</term><term>Viral</term><term>Virology</term><term>Virus particles</term><term>Wadell</term><term>Young children</term></keywords></textClass></profileDesc></teiHeader><front><div type="abstract" xml:lang="fr">The use of the polymerase chain reaction (PCR) for detection of human adenoviruses in diluted stool samples was investigated. Two sets of nested primers, including primers specific for the hexon‐coding region and for the E1 B region of enteric adenoviruses (EAd), were assessed by two‐step amplification. The primers constitute two different PCR systems designed for the detection of adenoviruses belonging to all six subgenera (A‐F), and the two EAds Ad40 and Ad41, respectively. In a two‐step PCR mediated amplification a single virus particle was detected when the two sets of general hexon primers or Ead specific primers were used. Earlier results from PCR detection of adenoviruses in stool from children suffering from diarrhea gave indications that adenovirus particles are commonly shed in stools without being identified as the cause of il I ness [Allard et a I.: Journal of Clinical Microbiology 28:2659‐2667, 1990]). Therefore, the general and the EAd specific PCR assays were assessed on 150 stool specimens from three groups including 50 healthy children, 50 healthy adults, and 50 adults suffering from diarrhea. When the two sets of general hexon primers were used, 25 of the 50 specimens from the healthy children (mean age 21 months) were found positive by two‐step PCR amplification. Nine of the 50 specimens from the healthy adults (mean age 32 years) were found positive whereas 12 of the 50 specimens from sick adults (mean age 31 years) gave amplification products, using the two sets of general hexon primers in a nested fashion. None of the 150 specimens were found to be positive by two‐step PCR amplification using the two sets of EAd‐specific primers. The sensitivity of the PCR, together with its simplicity and reduced time scale compared to other detection methods, support the potential of this technique as an additional method for routine detection of human adenovirus infections. © 1992 Wiley‐Liss, Inc.</div></front></TEI><affiliations><list><country><li>Suède</li></country></list><tree><country name="Suède"><noRegion><name sortKey="Allard, Annika" sort="Allard, Annika" uniqKey="Allard A" first="Annika" last="Allard">Annika Allard</name></noRegion><name sortKey="Albinsson, Bo" sort="Albinsson, Bo" uniqKey="Albinsson B" first="Bo" last="Albinsson">Bo Albinsson</name><name sortKey="Allard, Annika" sort="Allard, Annika" uniqKey="Allard A" first="Annika" last="Allard">Annika Allard</name><name sortKey="Wadell, Goran" sort="Wadell, Goran" uniqKey="Wadell G" first="Göran" last="Wadell">Göran Wadell</name></country></tree></affiliations></record>Pour manipuler ce document sous Unix (Dilib)
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