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In vitro experimental infection of primary duck hepatocyte cultures with duck hepatitis B virus.

机译:鸭乙肝病毒体外感染原代鸭肝细胞培养物。

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摘要

Duck hepatitis B virus (DHBV) obtained from the serum of congenitally infected ducks was used to infect primary duck hepatocyte cultures 1 to 4 days after plating. Virus replication was demonstrated by the appearance, beginning at 2 days after infection, of intracellular covalently closed-circular and single-stranded DHBV DNA replicative intermediates which were not present in the inoculating virus preparation. With increasing time after infection there was further amplification of intracellular relaxed circular, covalently closed-circular, and single-stranded DHBV DNA. Cultures of primary duck hepatocytes are competent for infection with DHBV only during the first 4 days of culture. Synthesis of DHBV core antigen and DHBV surface antigen was detected by immunofluorescence in 10% of the hepatocytes in culture. De novo synthesis and release of infectious virus was also demonstrated. Therefore, all stages of viral replication were carried out by these experimentally infected primary hepatocyte cultures. This system makes it possible to study DHBV replication in vitro.
机译:从先天感染鸭的血清中获得的鸭乙型肝炎病毒(DHBV)用于在接种后1-4天感染原代鸭肝细胞培养物。通过在感染后2天开始出现接种病毒制剂中不存在的细胞内共价闭环和单链DHBV DNA复制中间体来证明病毒复制。随着感染后时间的增加,细胞内松弛的环状,共价闭环和单链DHBV DNA进一步扩增。仅在培养的前4天,原代鸭肝细胞的培养才能够感染DHBV。通过免疫荧光法在培养的10%肝细胞中检测DHBV核心抗原和DHBV表面抗原的合成。从头开始合成和释放传染性病毒。因此,病毒复制的所有阶段都是通过这些实验感染的原代肝细胞培养物进行的。该系统使体外研究DHBV复制成为可能。

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