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In situ detection of hepatitis C virus RNA in liver tissue using a digoxigenin-labeled probe created during a polymerase chain reaction.

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dc.contributor.authorCho, SW-
dc.contributor.authorHwang, SG-
dc.contributor.authorHan, DC-
dc.contributor.authorJin, SY-
dc.contributor.authorLee, MS-
dc.contributor.authorShim, CS-
dc.contributor.authorLee, DW-
dc.contributor.authorLee, HB-
dc.date.accessioned2011-09-01T22:56:27Z-
dc.date.available2011-09-01T22:56:27Z-
dc.date.issued1996-
dc.identifier.issn0146-6615-
dc.identifier.urihttp://repository.ajou.ac.kr/handle/201003/3973-
dc.description.abstractThe cellular localization of hepatitis C virus (HCV) RNA in liver tissue was studied by nonisotopic in situ hybridization using a digoxigenin-labeled cDNA probe created during a polymerase chain reaction on samples from 16 patients with chronic HCV infection. Hybridization signals were recognized in the cytoplasm of the hepatocytes, and a few hepatocytes had hybridization signals in the nucleus as well. HCV RNA positive hepatocytes were found in 1 of 9 patients with chronic persistent hepatitis, 2 of 5 patients with chronic active hepatitis, and in each of 2 patients with chronic active hepatitis and cirrhosis. Positive signals were found in many hepatocytes within the lobule in liver sections of patients with advanced chronic active hepatitis. A number of HCV RNA positive hepatocytes were found in nodules, but not in the area of fibrosis. On the other hand, positive signals were found in a few hepatocytes scattered in the lobule in a patient with chronic persistent hepatitis. The mean ALT levels in the patients with positive signal (175.6 +/- 44.2 U/L) were significantly higher than in those without a signal (70.27 +/- 16.1 U/L) (P < 0.05). The findings suggest that a larger amount of HCV may be present during the advanced than during the early stages of type C hepatitis and nonisotopic in situ hybridization using a digoxigenin-labeled HCV cDNA probe created during a polymerase chain reaction deserves wider application for the detection of HCV replication in specimens.-
dc.formatapplication/pdf-
dc.language.isoen-
dc.subject.MESHAdult-
dc.subject.MESHAged-
dc.subject.MESHBase Sequence-
dc.subject.MESHColoring Agents-
dc.subject.MESHDNA Primers-
dc.subject.MESHDNA Probes-
dc.subject.MESHDNA, Viral-
dc.subject.MESHDigoxigenin-
dc.subject.MESHFemale-
dc.subject.MESHHepacivirus-
dc.subject.MESHHepatitis C-
dc.subject.MESHHumans-
dc.subject.MESHIn Situ Hybridization-
dc.subject.MESHLiver-
dc.subject.MESHMale-
dc.subject.MESHMiddle Aged-
dc.subject.MESHMolecular Sequence Data-
dc.subject.MESHPolymerase Chain Reaction-
dc.subject.MESHRNA, Viral-
dc.subject.MESHSensitivity and Specificity-
dc.titleIn situ detection of hepatitis C virus RNA in liver tissue using a digoxigenin-labeled probe created during a polymerase chain reaction.-
dc.typeArticle-
dc.identifier.pmid8801282-
dc.contributor.affiliatedAuthor조, 성원-
dc.type.localJournal Papers-
dc.identifier.doi10.1002/(SICI)1096-9071(199603)48:3<227::AID-JMV3>3.0.CO;2-A-
dc.citation.titleJournal of medical virology-
dc.citation.volume48-
dc.citation.number3-
dc.citation.date1996-
dc.citation.startPage227-
dc.citation.endPage233-
dc.identifier.bibliographicCitationJournal of medical virology, 48(3). : 227-233, 1996-
dc.identifier.eissn1096-9071-
dc.relation.journalidJ001466615-
Appears in Collections:
Journal Papers > School of Medicine / Graduate School of Medicine > Gastroenterology
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