New real-time-PCR method to identify single point mutations in hepatitis C virus

Chen, Qian; Belmonte, Irene; Buti, Marı́a; Nieto, Leonardo; García-Cehic, Damir; Gregori, Josep; Perales, Celia; Ordeig, Laura; Llorens-Revull, Meritxell; Soria, María Eugenia; Esteban, Rafael; Esteban, Juan Ignacio; Rodríguez‐Frías, Francisco; Quer, Josep

doi:10.3748/wjg.v22.i43.9604

Cited by 5 publications

(3 citation statements)

References 16 publications

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“…These data will further benefit our understanding of the relationship between env quasispecies and virulence. Firstly, we adopted double-probe real-time PCR to accurately determine the proportion of strains with the env -Δ236D-phenotype and env -236D-phenotype sequences (which refer to virus sequences without and with the 236D mutation) in different EIAV generations [23,24]. An env -236D-phenotype-specific probe (HEX) and an env -Δ236D-phenotype-specific probe (FAM) were designed based on the V4 domain sequences (Figure S2).…”

Section: Resultsmentioning

confidence: 99%

Characterization of EIAV env Quasispecies during Long-Term Passage In Vitro: Gradual Loss of Pathogenicity

Lin

Wang

et al. 2019

Viruses

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As the only widely used live lentiviral vaccine, the equine infectious anima virus (EIAV) attenuated vaccine was developed by in vitro passaging of a virulent strain for 121 generations. In our previous study, we observed that the attenuated vaccine was gradually selected under increased environmental pressure at the population level (termed a quasispecies). To further elucidate the potential correlation between viral quasispecies evolution and pathogenesis, a systematic study was performed by sequencing env using several methods. Some key mutations were identified within Env, and we observed that increased percentages of these mutations were accompanied by an increased passage number and attenuated virulence. Phylogenetic analysis revealed that env mutations related to the loss of virulence might have occurred evolutionarily. Among these mutations, deletion of amino acid 236 in the V4 region of Env resulted in the loss of one N-glycosylation site that was crucial for virulence. Notably, the 236-deleted sequence represented a “vaccine-specific” mutation that was also found in wild EIAVLN40 strains based on single genome amplification (SGA) analysis. Therefore, our results suggest that the EIAV attenuated vaccine may originate from a branch of quasispecies of EIAVLN40. Generally, the presented results may increase our understanding of the attenuation mechanism of the EIAV vaccine and provide more information about the evolution of other lentiviruses.

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Section: Resultsmentioning

confidence: 99%

Characterization of EIAV env Quasispecies during Long-Term Passage In Vitro: Gradual Loss of Pathogenicity

Lin

Wang

et al. 2019

Viruses

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“…In clinical diagnostic virology and epidemiology, multiplex polymerase chain reaction (mPCR) and mRT-PCR have been widely used for identifying genotypes and detecting mutations. For example, Hepatitis C virus variants with a single nucleotide change or multiple nucleotide changes are well characterized by mRT-PCR [ 4 ]. The use of human papilloma virus (HPV) genotype sequence-specific PCR primers/probes allows for the amplification of the target viral gene only if the target DNA remains in the specimens.…”

Section: Introductionmentioning

confidence: 99%

SARS-CoV-2 Continuous Genetic Divergence and Changes in Multiplex RT-PCR Detection Pattern on Positive Retesting Median 150 Days after Initial Infection

Liu

Rodriguez

Zhou

et al. 2022

IJMS

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Being in the epicenter of the COVID-19 pandemic, our lab tested 193,054 specimens for SARS-CoV-2 RNA by diagnostic multiplex reverse transcription polymerase chain reaction (mRT-PCR) starting in March 2020, of which 17,196 specimens resulted positive. To investigate the dynamics of virus molecular evolution and epidemiology, whole genome amplification (WGA) and Next Generation Sequencing (NGS) were performed on 9516 isolates. 7586 isolates with a high quality were further analyzed for the mutation frequency and spectrum. Lastly, we evaluated the utility of the mRT-PCR detection pattern among 26 reinfected patients with repeat positive testing three months after testing negative from the initial infection. Our results show a continuation of the genetic divergence in viral genomes. Furthermore, our results indicate that independent mutations in the primer and probe regions of the nucleocapsid gene amplicon and envelope gene amplicon accumulate over time. Some of these mutations correlate with the changes of detection pattern of viral targets of mRT-PCR. Our data highlight the significance of a continuous genetic divergence on a gene amplification-based assay, the value of the mRT-PCR detection pattern for complementing the clinical diagnosis of reinfection, and the potential for WGA and NGS to identify mutation hotspots throughout the entire viral genome to optimize the design of the PCR-based gene amplification assay.

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“…This approach has become an invaluable tool in the analysis of SNS in the human genome 1 and distinguishing drug resistant from drug susceptible bacterial strains, 2 but has often failed in the analysis of viral sequences. 3 Indeed, viral genomes are particularly prone to mutations, due to the absence of the proofreading activities of viral nucleic acid polymerases, a strategy that enables escape from the immune system and the rapid development of drug resistance. 4 This makes the frequent need to differentiate between two closely related viral species even more complicated.…”

mentioning

confidence: 99%

A mutation-resistant deoxyribozyme OR gate for highly selective detection of viral nucleic acids

et al. 2017

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Highly selective probes hybridize only to fully complementary DNA or RNA sequences and, therefore, often fail to recognize mutated viral genomes. Here we designed a probe that possesses two seemingly incompatible properties: it tolerates some point mutations in genome, while it remains selective towards others. An OR deoxyribozyme logic gate was designed to fluorescently report the sequences of enterovirus 71 (EV71) covering ~90% of all known EV71 strains. Importantly, sequences of closely related coxsackieviruses that differed by single nucleotides were reliably differentiated in 7 out of 8 cases.

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New real-time-PCR method to identify single point mutations in hepatitis C virus

Cited by 5 publications

References 16 publications

Characterization of EIAV env Quasispecies during Long-Term Passage In Vitro: Gradual Loss of Pathogenicity

Characterization of EIAV env Quasispecies during Long-Term Passage In Vitro: Gradual Loss of Pathogenicity

SARS-CoV-2 Continuous Genetic Divergence and Changes in Multiplex RT-PCR Detection Pattern on Positive Retesting Median 150 Days after Initial Infection

A mutation-resistant deoxyribozyme OR gate for highly selective detection of viral nucleic acids

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