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荧光单链构象多态性分析丙型肝炎病毒感染中的准种

Quasispecies analysis in hepatitis C virus infection by fluorescent single strand conformation polymorphism.

作者信息

Peters T, Schlayer H J, Hiller B, Rösler B, Blum H, Rasenack J

机构信息

University Hospital, Department of Medicine II, Freiburg, Germany.

出版信息

J Virol Methods. 1997 Feb;64(1):95-102. doi: 10.1016/s0166-0934(96)02144-1.

Abstract

Hepatitis C virus (HCV) results frequently in chronic hepatitis and its sequelae liver cirrhosis and hepatocellular carcinoma. Interferon-alpha is at present the most effective treatment, resulting in a sustained response in about 20-25% of patients. HCV genotype, titer and quasispecies determine the success of treatment. In this study, fluorescent single strand conformation polymorphism (f-SSCP) was evaluated for the analysis of HCV quasispecies. Two sera from a chronically HCV-infected patient, obtained 6 years apart, were examined. The hypervariable region I (HVRI) of the HCV genome was amplified by reverse transcription and PCR. The PCR products were cloned and sequenced or fluorescein-labeled and subjected to f-SSCP. Both methods demonstrated a single HCV species in the early serum and multiple quasispecies in the late serum. Single clones of the heterogeneous virus population were used to optimize conditions for f-SSCP. The most important factors were the gel temperature and virus titer. At the optimal running temperature one base exchange in 218 bases was detectable. Repeat extractions and amplifications gave identical results. Dilution of the serum containing multiple quasispecies resulted in a 'loss' of species. Provided the running temperature is optimal and virus titer is sufficient, f-SSCP is shown to be fast and reliable for HCV quasispecies analysis.

摘要

丙型肝炎病毒(HCV)常常导致慢性肝炎及其后遗症肝硬化和肝细胞癌。目前,α干扰素是最有效的治疗方法,约20%-25%的患者会出现持续应答。HCV基因型、滴度和准种决定治疗的成败。在本研究中,对荧光单链构象多态性(f-SSCP)用于分析HCV准种进行了评估。检测了一名慢性HCV感染患者相隔6年采集的两份血清。通过逆转录和PCR扩增HCV基因组的高变区I(HVR1)。PCR产物进行克隆和测序,或用荧光素标记后进行f-SSCP分析。两种方法均显示早期血清中为单一HCV毒株,晚期血清中有多个准种。利用异质病毒群体的单个克隆优化f-SSCP条件。最重要的因素是凝胶温度和病毒滴度。在最佳运行温度下,可检测到218个碱基中有一个碱基发生交换。重复提取和扩增得到相同结果。含有多个准种的血清稀释会导致毒株“丢失”。如果运行温度最佳且病毒滴度足够,f-SSCP对HCV准种分析而言快速且可靠。

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