2010
DOI: 10.1128/jvi.02698-09
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Development of an Intergenotypic Hepatitis C Virus (HCV) Cell Culture Method To Assess Antiviral Susceptibilities and Resistance Development of HCV NS3 Protease Genes from HCV Genotypes 1 to 6

Abstract: Protease inhibitors (PIs) of hepatitis C virus (HCV) provide an additional or alternative therapy for chronic infection. However, assessment of their efficacy and ability to inhibit replication of different genotypes is hampered by the lack of a convenient animal model or a method for in vitro culture of HCV other than the type 1/2-based replicons and the infectious genotype 2a clone JFH1. To address this problem, we constructed a panel of replication-competent chimeric Jc1 (pFK JFH1/J6/C-846) clones containin… Show more

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Cited by 33 publications
(58 citation statements)
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References 64 publications
(87 reference statements)
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“…Synthesis of cDNA via gene specific primer reverse transcription (GSP-RT) was performed using Superscript III Reverse transcriptase (Life Technologies) according to the manufacturer's instructions, with minor modifications. 8µl of extracted vRNA was used for GSP-RT in 20µl volumes using 2pmol primer (5'-TCYGCTTGGTCMAGGAC-3') (Imhof and Simmonds, 2010). Reverse transcription reactions were incubated at 50C for 1 hour followed by 42C for 1 hour.…”
Section: Amplification Of Hcv Ns3 Protease Domainmentioning
confidence: 99%
See 1 more Smart Citation
“…Synthesis of cDNA via gene specific primer reverse transcription (GSP-RT) was performed using Superscript III Reverse transcriptase (Life Technologies) according to the manufacturer's instructions, with minor modifications. 8µl of extracted vRNA was used for GSP-RT in 20µl volumes using 2pmol primer (5'-TCYGCTTGGTCMAGGAC-3') (Imhof and Simmonds, 2010). Reverse transcription reactions were incubated at 50C for 1 hour followed by 42C for 1 hour.…”
Section: Amplification Of Hcv Ns3 Protease Domainmentioning
confidence: 99%
“…Nested PCR was performed using previously described 1a-specific primer pairs (Imhof and Simmonds, 2010).…”
Section: Amplification Of Hcv Ns3 Protease Domainmentioning
confidence: 99%
“…Huh7.5 cells (3.5 ϫ 10 5 /well) were plated in a 6-well plate, incubated overnight, and infected with stocks of HCV genotype 1 to 6 recombinants for 24 h. PIs purchased from Acme Bioscience were dissolved in dimethyl sulfoxide (Sigma) (21,28 50 of faldaprevir (BI 201335), paritaprevir (ABT-450), or deldeprevir (ACH-2684) was initiated when ϳ1% to 20% cells were infected. Cultures were retreated with the PI upon cell splitting every 2 to 3 days; cells plated on a chamber slide after treatment and incubated overnight were immunostained as described above in order to evaluate viral spread.…”
Section: Methodsmentioning
confidence: 99%
“…Several enzymatic and replicon-based phenotypic assays have been developed for assessing the PI susceptibilities of HCV through replicons with NS3 genes derived from clinical isolates (17)(18)(19) or recombinant NS3 proteases coded by the NS3 genes of HCV in patient sera (13). These assays can confirm the effects of new mutations or complex mutation patterns on HCV susceptibility to protease inhibitors, but they are laborious and time-consuming, with turnaround times ranging from a few days to weeks.…”
mentioning
confidence: 99%