Viral Sequence Evolution in Acute Hepatitis C Virus Infection

Kuntzen, Thomas; Timm, Joerg; Berical, Andrew; Lewis-Ximenez, Lia Laura; Jones, Andrea M.; Nolan, Brian E.; Wiesch, Julian Schulze zur; Li, Bin; Schneidewind, Arne; Kim, Arthur Y.; Chung, Raymond T.; Lauer, Georg M.; Allen, Todd M.

doi:10.1128/jvi.00995-07

Cited by 96 publications

(143 citation statements)

References 54 publications

(84 reference statements)

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“…For autologous virus sequencing, viral RNA was extracted from plasma samples using the vRNA extraction kit (Qiagen). A nested PCR with 12 external and 36 internal primer pairs spanning the entire HCV coding sequence amplified overlapping fragments of approximately 500-1.2 kb, as previously described (48). PCR fragments were then purified (PCR Purification Kit; Qiagen) and population sequenced bidirectionally on an ABI 3730 PRISM automated sequencer (48).…”

Section: Figurementioning

confidence: 99%

Tim-3 expression on PD-1+ HCV-specific human CTLs is associated with viral persistence, and its blockade restores hepatocyte-directed in vitro cytotoxicity

McMahan

Golden-Mason²,

Nishimura³

et al. 2010

J. Clin. Invest.

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276

248

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Having successfully developed mechanisms to evade immune clearance, hepatitis C virus (HCV) establishes persistent infection in approximately 75%-80% of patients. In these individuals, the function of HCV-specific CD8 + T cells is impaired by ligation of inhibitory receptors, the repertoire of which has expanded considerably in the past few years. We hypothesized that the coexpression of the negative regulatory receptors T cell immunoglobulin and mucin domain-containing molecule 3 (Tim-3) and programmed death 1 (PD-1) in HCV infection would identify patients at risk of developing viral persistence during and after acute HCV infection. The frequency of PD-1 -Tim-3 -HCV-specific CTLs greatly outnumbered PD-1 + Tim-3 + CTLs in patients with acute resolving infection. Moreover, the population of PD-1 + Tim-3 + T cells was enriched for within the central memory T cell subset and within the liver. Blockade of either PD-1 or Tim-3 enhanced in vitro proliferation of HCV-specific CTLs to a similar extent, whereas cytotoxicity against a hepatocyte cell line that expressed cognate HCV epitopes was increased exclusively by Tim-3 blockade. These results indicate that the coexpression of these inhibitory molecules tracks with defective T cell responses and that anatomical differences might account for lack of immune control of persistent pathogens, which suggests their manipulation may represent a rational target for novel immunotherapeutic approaches.

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Section: Figurementioning

confidence: 99%

Tim-3 expression on PD-1+ HCV-specific human CTLs is associated with viral persistence, and its blockade restores hepatocyte-directed in vitro cytotoxicity

McMahan

Golden-Mason²,

Nishimura³

et al. 2010

J. Clin. Invest.

Self Cite

276

248

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“…In an infected individual, serum HCV RNA levels can reach 10 to 100 million IU/ml (40). The viral RNA polymerase is estimated to make 1 error per 10,000 to 100,000 bp copied (22), but the viral genome is only 9,600 bases, resulting in diversification of the viral population, so that most viral genomes differ in sequence from the population consensus (16,20,21). Thus, when antiviral pressure is exerted on a viral population, sequence variants with reduced sensitivity may expand in the presence of the selective pressure (30, 41) and cause resistance (37).…”

mentioning

confidence: 99%

Hepatitis C Virus Transmission Bottlenecks Analyzed by Deep Sequencing

Wang

Sherrill-Mix

Chang

et al. 2010

J Virol

136

135

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Hepatitis C virus (HCV) replication in infected patients produces large and diverse viral populations, which give rise to drug-resistant and immune escape variants. Here, we analyzed HCV populations during transmission and diversification in longitudinal and cross-sectional samples using 454/Roche pyrosequencing, in total analyzing 174,185 sequence reads. To sample diversity, four locations in the HCV genome were analyzed, ranging from high diversity (the envelope hypervariable region 1 [HVR1]) to almost no diversity (the 5 untranslated region [UTR]). For three longitudinal samples for which early time points were available, we found that only 1 to 4 viral variants were present, suggesting that productive infection was initiated by a very small number of HCV particles. Sequence diversity accumulated subsequently, with the 5 UTR showing almost no diversification while the envelope HVR1 showed >100 variants in some subjects. Calculation of the transmission probability for only a single variant, taking into account the measured population structure within patients, confirmed initial infection by one or a few viral particles. These findings provide the most detailed sequence-based analysis of HCV transmission bottlenecks to date. The analytical methods described here are broadly applicable to studies of viral diversity using deep sequencing.Hepatitis C virus (HCV) is a positive-strand enveloped RNA virus of the flavivirus family. HCV infects ϳ170 million people worldwide with a high rate of persistence (1, 2) and is a major etiological agent of chronic hepatitis, liver cirrhosis, and hepatocellular carcinoma. The current standard of therapy is the combined use of pegylated alpha interferon (IFN-␣) and ribavirin (9), although there are substantial limitations due to toxicity and resistance profiles (47). Recent development of various small-molecule inhibitors that specifically target HCV offer some promise (13), but challenges still remain because the size and diversity of viral populations promote rapid development of drug resistance (28,42). In an infected individual, serum HCV RNA levels can reach 10 to 100 million IU/ml (40). The viral RNA polymerase is estimated to make 1 error per 10,000 to 100,000 bp copied (22), but the viral genome is only 9,600 bases, resulting in diversification of the viral population, so that most viral genomes differ in sequence from the population consensus (16,20,21). Thus, when antiviral pressure is exerted on a viral population, sequence variants with reduced sensitivity may expand in the presence of the selective pressure (30, 41) and cause resistance (37). Consistent with this, differential sequence diversity in HCV populations has been linked to clinical outcome (7,8).The size and complexity of HCV populations has made their analysis challenging. However, new deep-sequencing and bioinformatics methods are well suited to analyzing this problem. Using the 454/Roche technology, it is possible to generate more than 10 8 bases of DNA sequence in a single 1-day run, albeit in fragments...

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“…RT-PCR was performed using the RNA reaction mixture (18 µl) containing 4 U of RNAsin, 0.27 µM of each forward and reverse primers (HCV 5UT F and R, Cha et al, 1992) [13][14] , and 15 µl of viral RNA, was prepared. The RNA mix was incubated for 5 minutes at 65 0 C and 10 minutes at room temperature.…”

Section: In-house Rt-pcr Assay For the Detection Of Hcvmentioning

confidence: 99%

Automated Low Cost Method of Quantification of Hepatitis C Virus

Marikar

Senevirathna

Fernandopulle

2015

Bangladesh J Med Sci

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Abstract:This paper describes the development of a Dig-dUTP based multiplex real time RT-PCR for the simultaneous detection of HCV viral amount in plasma samples. Viral genomes were identified in the same sample by Dig-dUTP PCR 216 bp region. Analysis of known scalar concentrations of reference plasma indicated that the multiplex procedure detects at least 500 copies/ml of HCV. In addition, we also assayed HCV viral load in eighty co-infected patients and in fifteen blood donors, confirming the sensitivity and specificity of the assay. This method may represent a useful alternative method for the detection of HCV co-infection, reliable for a rapid and relatively inexpensive screening of blood donors. The assay may be used to determine posttherapy viral clearance.

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Viral Sequence Evolution in Acute Hepatitis C Virus Infection

Cited by 96 publications

References 54 publications

Tim-3 expression on PD-1+ HCV-specific human CTLs is associated with viral persistence, and its blockade restores hepatocyte-directed in vitro cytotoxicity

Tim-3 expression on PD-1+ HCV-specific human CTLs is associated with viral persistence, and its blockade restores hepatocyte-directed in vitro cytotoxicity

Hepatitis C Virus Transmission Bottlenecks Analyzed by Deep Sequencing

Automated Low Cost Method of Quantification of Hepatitis C Virus

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