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Quantitative measurement of Hepatitis B virus cccDNA

机译:乙肝病毒cccDNA的定量检测

摘要

Hepatitis B Virus (HBV) infection results in the entry of viral genomic DNA into host liver cells. This viral relaxed circular DNA (rcDNA) is transported into the nucleus and converted into covalent closed-circular DNA (cccDNA), which serves as a template for viral transcription. Elimination of cccDNA is needed to cure HBV infection, which remains a major therapeutic challenge. A robust and sensitive method to measure cccDNA described here is useful to facilitate drug development and to monitor efficacy of therapy. A set of primers were designed in combination with sodium bisulfite treatment of viral DNA, allowing specific amplification of cccDNA without interfering amplification of rcDNA. This method can be used to further guide therapeutic development, and to provide a non-invasive alternative to monitoring of HBV-infected patients undergoing antiviral treatments.
机译:乙型肝炎病毒(HBV)感染导致病毒基因组DNA进入宿主肝细胞。这种病毒松弛的环状DNA(rcDNA)被转运到细胞核中,并转化为共价的封闭环状DNA(cccDNA),作为病毒转录的模板。需要消除cccDNA才能治愈HBV感染,这仍然是主要的治疗挑战。本文所述的一种可靠而灵敏的测量cccDNA的方法可用于促进药物开发和监测治疗效果。设计了一套引物,结合亚硫酸氢钠处理病毒DNA,可以特异性扩增cccDNA,而不会干扰rcDNA的扩增。该方法可用于进一步指导治疗的发展,并为监测正在接受抗病毒治疗的HBV感染患者提供无创替代方法。

著录项

  • 公开/公告号US2017233832A1

    专利类型

  • 公开/公告日2017-08-17

    原文格式PDF

  • 申请/专利权人 JBS SCIENCE INC.;

    申请/专利号US201715433839

  • 发明设计人 SURBHI JAIN;JAMIN DEAN STEFFEN;WEI SONG;

    申请日2017-02-15

  • 分类号C12Q1/70;G01N21/64;C12Q1/68;

  • 国家 US

  • 入库时间 2022-08-21 13:51:54

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