Dynamics of Hepatitis B Virus Quasispecies in Association with Nucleos(t)ide Analogue Treatment Determined by Ultra-Deep Sequencing

Nishijima, Norihiro; Marusawa, Hiroyuki; Ueda, Yoshihide; Takahashi, Ken; Nasu, Akihiro; Osaki, Yukio; Kou, Tadayuki; Yazumi, Shujiro; Fujiwara, Takeshi; Tsuchiya, Soken; Shimizu, Kazuharu; Üemoto, Shinji; Chiba, Tsutomu

doi:10.1371/journal.pone.0035052

Cited by 71 publications

(69 citation statements)

References 37 publications

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“…Although it was difficult to detect a small population of variants in the host genome using a traditional approach such as PCR, NGS, owing to its depth, enabled us to detect a novel genomic variation (27). NGS has strongly supported the studies of viral genetic diversity, especially in RNA viruses (28,29), whereas the detection by NGS of quasispecies in DNA virus has been reported less frequently (30)(31)(32)(33). Using PCR analysis, the presence of VP1 quasispecies has been reported in polyomavirus BK (BKV) (34).…”

Section: Discussionmentioning

confidence: 99%

Deep-Sequence Identification and Role in Virus Replication of a JC Virus Quasispecies in Patients with Progressive Multifocal Leukoencephalopathy

Takahashi

Sekizuka

Fukumoto

et al. 2017

J Virol

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JC virus (JCV) is a DNA virus causing progressive multifocal leukoencephalopathy (PML) in immunodeficient patients. In the present study, 22 genetic quasispecies with more than 1.5% variant frequency were detected in JCV genomes from six clinical samples of PML by next-generation sequencing. A mutation from A to C at nucleotide (nt) 3495 in JCV Mad1 resulting in a V-to-G amino acid substitution at amino acid (aa) position 392 of the large T antigen (TAg) was identified in all six cases of PML at 3% to 19% variant frequencies. Transfection of JCV Mad1 DNA possessing the V392G substitution in TAg into IMR-32 and human embryonic kidney 293 (HEK293) cells resulted in dramatically decreased production of JCV-encoded proteins. The virus DNA copy number was also reduced in supernatants of the mutant virus-transfected cells. Transfection of the IMR-32 and HEK293 cells with a virus genome containing a revertant mutation recovered viral production and protein expression. Cotransfection with equal amounts of wild-type genome and mutated JCV genome did not reduce the expression of viral proteins or viral replication, suggesting that the mutation did not have any dominantnegative function. Finally, immunohistochemistry demonstrated that TAg was expressed in all six pathological samples in which the quasispecies were detected. In conclusion, the V392G amino acid substitution in TAg identified frequently in PML lesions has a function in suppressing JCV replication, but the frequency of the mutation was restricted and its role in PML lesions was limited.IMPORTANCE DNA viruses generally have lower mutation frequency than RNA viruses, and the detection of quasispecies in JCV has rarely been reported. In the present study, a next-generation sequencer identified a JCV quasispecies with an amino acid substitution in the T antigen in patients with PML. In vitro studies showed that the mutation strongly repressed the expression of JC viral proteins and reduced the viral replication. However, because the frequency of the mutation was low in each case, the total expression of virus proteins was sustained in vivo. Thus, JC virus replicates in PML lesions in the presence of a mutant virus which is able to repress virus replication.

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Section: Discussionmentioning

confidence: 99%

Deep-Sequence Identification and Role in Virus Replication of a JC Virus Quasispecies in Patients with Progressive Multifocal Leukoencephalopathy

Takahashi

Sekizuka

Fukumoto

et al. 2017

J Virol

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“…Massively-parallel sequencing was performed as described previously 19,20 . Fragmented DNA (>5 µg) was used to prepare each DNA sequencing library.…”

Section: Methodsmentioning

confidence: 99%

Accumulation of Somatic Mutations in TP53 in Gastric Epithelium With Helicobacter pylori Infection

et al. 2014

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“…The heterogeneity of viral quasispecies was evaluated by a complexity metric based on the number of variants and their prevalence detected in the population. Quasispecies complexity at the aa and nt level was estimated for each site using S n according to the following formula: S n 52S i ( f i lnf i ), where f i represents the frequency of a particular variant in the quasispecies (Domingo et al, 2006;Nishijima et al, 2012). The mean viral complexity in each sample was determined by calculating the total S n at each position and dividing by the total length nt or aa number.…”

Section: Methodsmentioning

confidence: 99%

“…In the previous studies, the quasispecies were detected by direct PCR sequencing and the variants in complexity were defined based on the whole length of the reads (Chen et al, 2009;Liu et al, 2011). However, in our study, the complexity was measured by the mean Shannon entropy (S n ) at each nt or aa position following the methods reported previously (Nishijima et al, 2012); (2) the time point of sampling. The quasispecies may show different patterns of evolution at different stages of therapy; (3) different drugs used in the therapy.…”

Section: Resistant Mutations and Hbv Quasispecies In Ldt Therapymentioning

confidence: 99%

Resistant mutations and quasispecies complexity of hepatitis B virus during telbivudine treatment

Yin

Wei

et al. 2015

Journal of General Virology

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Ultra-deep pyrosequencing (UDPS) was used to analyse the dynamics of quasispecies and resistant mutations during telbivudine (LDT) treatment of hepatitis B patients. Twenty-six HBeAg-positive chronic hepatitis B patients were treated with LDT for a period of 104 weeks and were characterized as 16 responders, six partial responders and four viral breakthrough patients based on hepatitis B virus (HBV) DNA levels. The plasma samples were subjected to UDPS of the reverse transcriptase (RT) region of HBV. Mutations rtM204I, rtL80I and rtL80V were detected in at least three of the four viral breakthrough patients, indicating the significant roles of the mutations in resistance to LDT. The degree of complexity of viral quasispecies remained in a steady state in the absence of selection pressure, but increased after the LDT treatment. The complexity in the responder group at week 12 was significantly higher than that in the group comprising partial responders and viral breakthrough patients. In vitro replication efficiency analyses showed that the RT mutations had different impacts on HBV replication, with a tendency of rtM204I.rtL80V.rtL80I. Furthermore, double mutations rtL80I/M204I and rtL80V/M204V had replication efficiency similar to that of rtL80I and rtL80V, respectively. Consistent with previous studies, mutation rtM204I was found to be highly resistant to LDT. However, in contrast with their sensitivity to lamivudine, rtL80I and rtL80V were moderately resistant to LDT. Our results indicated that rtL80I and rtL80V may not only serve as replication complementary mutations to rtM204I, but also directly contribute to the LDT resistance.

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Dynamics of Hepatitis B Virus Quasispecies in Association with Nucleos(t)ide Analogue Treatment Determined by Ultra-Deep Sequencing

Cited by 71 publications

References 37 publications

Deep-Sequence Identification and Role in Virus Replication of a JC Virus Quasispecies in Patients with Progressive Multifocal Leukoencephalopathy

Deep-Sequence Identification and Role in Virus Replication of a JC Virus Quasispecies in Patients with Progressive Multifocal Leukoencephalopathy

Accumulation of Somatic Mutations in TP53 in Gastric Epithelium With Helicobacter pylori Infection

Resistant mutations and quasispecies complexity of hepatitis B virus during telbivudine treatment

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