2016
DOI: 10.1016/j.bjm.2016.07.008
|View full text |Cite
|
Sign up to set email alerts
|

In-house quantitative real-time PCR for the diagnosis of hepatitis B virus and hepatitis C virus infections

Abstract: The quantification of viral nucleic acids in serum by real-time PCR plays an important role in diagnosing hepatitis B virus and hepatitis C virus infection. In this study, we developed an assay using specific primers and probes to quantify hepatitis B virus DNA or hepatitis C virus RNA in serum from infected patients. For standardization and validation of the assay, an international panel of hepatitis B virus/hepatitis C virus and standard plasmids was used. A correlation coefficient of 0.983 and 0.963 for hep… Show more

Help me understand this report

Search citation statements

Order By: Relevance

Paper Sections

Select...
2
1
1
1

Citation Types

0
5
0

Year Published

2017
2017
2024
2024

Publication Types

Select...
7
1

Relationship

0
8

Authors

Journals

citations
Cited by 10 publications
(5 citation statements)
references
References 20 publications
0
5
0
Order By: Relevance
“…Cycle threshold (Ct) and viral load correlation q-PCR results, including Ct values, were obtained from the computerized Central Virology Laboratory database. Extrapolation of the adenoviral load from Ct was calculated using known quantitated samples as a reference, a common method for quantifying viral load in clinical samples (Borg et al, 2003;Zauli et al, 2016). For adenovirus DNA copy number calibration, samples with predetermined copy numbers provided by the Quality Control for Molecular Diagnostics (QCMD) were used.…”
Section: Viral Genome Quantification By Real-time Pcr (Q-pcr)mentioning
confidence: 99%
“…Cycle threshold (Ct) and viral load correlation q-PCR results, including Ct values, were obtained from the computerized Central Virology Laboratory database. Extrapolation of the adenoviral load from Ct was calculated using known quantitated samples as a reference, a common method for quantifying viral load in clinical samples (Borg et al, 2003;Zauli et al, 2016). For adenovirus DNA copy number calibration, samples with predetermined copy numbers provided by the Quality Control for Molecular Diagnostics (QCMD) were used.…”
Section: Viral Genome Quantification By Real-time Pcr (Q-pcr)mentioning
confidence: 99%
“…Quantitative PCR (qPCR)-based assays have routinely been used for the detection of hepatitis B virus and hepatitis C virus [41]. There is no report of any quantification assay for detection of any PVT1-derived transcripts.…”
Section: Discussionmentioning
confidence: 99%
“…The observed false positive results, hence, higher HCV antibody seroprevalence (1.67%) by Diaspot rapid enzyme immunoassay compared to that of Biorad Genscreen HCV Ag-Ab Monolisa assay (0.33%) based on 'sandwich' ELISA technique in this study contrast the outcomes of studies by other researchers who found false negative results using Diaspot rapid one-step enzyme immunoassay [18] . Current trends in transfusion service demand that initial screening of blood and blood products be based on ELISA technique using kit that both screen for the HCV core antigen and anti-HCV antibodies that improves early detection of HCV infection during the window period and subsequent confirmation of HCV status with recombinant immunoblotting assay (RIBA) or nucleic acid testing (NAT) by real-time PCR [40][41][42] . Literatures have showed that continued development of newer testing techniques have helped to significantly improve early detection and reduce the window period from 82 days to 66 days and even lower [43] .…”
Section: Discussionmentioning
confidence: 99%