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利用链特异性逆转录/聚合酶链反应证明丙型肝炎病毒对黑猩猩肝细胞的体外感染

Demonstration of in vitro infection of chimpanzee hepatocytes with hepatitis C virus using strand-specific RT/PCR.

作者信息

Lanford R E, Sureau C, Jacob J R, White R, Fuerst T R

机构信息

Department of Virology and Immunology, Southwest Foundation for Biomedical Research, San Antonio, Texas 78228.

出版信息

Virology. 1994 Aug 1;202(2):606-14. doi: 10.1006/viro.1994.1381.

Abstract

Analysis of hepatitis C virus (HCV) replication has been hampered due to the difficulty encountered in in vitro cultivation of the virus in conventional tissue culture systems. In this study, primary chimpanzee hepatocyte cultures maintained in a serum-free medium formulation were susceptible to in vitro infection with HCV. In order to document infection, two new methods of reverse transcription/polymerase chain reaction were developed that permit accurate distinction between positive and negative strand HCV RNA. One method relied upon the use of a tagged cDNA primer, while the second method employed a thermostable reverse transcriptase. Following inoculation of chimpanzee hepatocytes with HCV, intracellular positive and negative strand HCV RNA were detectable 4 days postinfection and throughout the remainder of the experimental period, 25 days. Analysis of HCV-inoculated baboon hepatocytes revealed a total absence of negative strand HCV RNA, while residual positive strand RNA from the inoculum could be detected for up to 11 days. The in vitro replication of HCV RNA in chimpanzee hepatocytes could be suppressed by alpha-interferon. This system should be amenable to the study of HCV replication, antiviral compounds, and the development of neutralization assays.

摘要

由于在传统组织培养系统中体外培养丙型肝炎病毒(HCV)存在困难,HCV复制的分析受到了阻碍。在本研究中,在无血清培养基配方中维持的原代黑猩猩肝细胞培养物易受HCV的体外感染。为了记录感染情况,开发了两种新的逆转录/聚合酶链反应方法,可准确区分HCV RNA的正链和负链。一种方法依赖于使用标记的cDNA引物,而第二种方法使用热稳定逆转录酶。用HCV接种黑猩猩肝细胞后,感染后4天及整个实验期(25天)内均可检测到细胞内正链和负链HCV RNA。对接种HCV的狒狒肝细胞的分析显示完全没有负链HCV RNA,而接种物中的残留正链RNA最多可检测11天。α-干扰素可抑制HCV RNA在黑猩猩肝细胞中的体外复制。该系统应适用于HCV复制、抗病毒化合物的研究以及中和试验的开发。

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