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Detection of HBV Covalently Closed Circular DNA

机译:HBV共价闭合环状DNA的检测

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Chronic hepatitis B virus (HBV) infection affects approximately 240 million people worldwide and remains a serious public health concern because its complete cure is impossible with current treatments. Covalently closed circular DNA (cccDNA) in the nucleus of infected cells cannot be eliminated by present therapeutics and may result in persistence and relapse. Drug development targeting cccDNA formation and maintenance is hindered by the lack of efficient cccDNA models and reliable cccDNA detection methods. Southern blotting is regarded as the gold standard for quantitative cccDNA detection, but it is complicated and not suitable for high-throughput drug screening, so more sensitive and simple methods, including polymerase chain reaction (PCR)-based methods, Invader assays, in situ hybridization and surrogates, have been developed for cccDNA detection. However, most methods are not reliable enough, and there are no unified standards for these approaches. This review will summarize available methods for cccDNA detection. It is hoped that more robust methods for cccDNA monitoring will be developed and that standard operation procedures for routine cccDNA detection in scientific research and clinical monitoring will be established.
机译:慢性乙型肝炎病毒(HBV)感染影响全球约2.4亿人,并且仍然是严重的公共卫生问题,因为用目前的治疗方法无法完全治愈。目前的治疗方法无法消除感染细胞核中共价闭合的环状DNA(cccDNA),并可能导致持久性和复发。缺乏有效的cccDNA模型和可靠的cccDNA检测方法阻碍了针对cccDNA形成和维持的药物开发。 Southern印迹法被认为是定量cccDNA检测的金标准,但是它很复杂且不适合高通量药物筛选,因此更灵敏,更简单的方法,包括基于聚合酶链反应(PCR)的方法,Invader检测,原位检测已经开发出杂交和替代物用于cccDNA检测。但是,大多数方法不够可靠,并且这些方法还没有统一的标准。这篇评论将总结cccDNA检测的可用方法。希望能开发出更可靠的cccDNA监测方法,并建立科学研究和临床监测中常规cccDNA检测的标准操作程序。

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