首页> 外文期刊>Journal of Medical Virology >293 cells over-expressing human ADI1 and CD81 are permissive for serum-derived hepatitis C virus infection.
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293 cells over-expressing human ADI1 and CD81 are permissive for serum-derived hepatitis C virus infection.

机译:过量表达人ADI1和CD81的293细胞可用于血清源性丙型肝炎病毒感染。

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摘要

Human aci-reductone dioxygenase 1 (ADI1) is a member of the Cupin superfamily. It binds to and inhibits the activities of membrane-type 1 matrix metalloproteinase, a protein known to interact with the tight junction protein, claudin-1. Previously, a variant protein, named submergence-induced protein-like factor (Sip-L), consisting of ADI1 amino acids 64-179, was found to support hepatitis C virus (HCV) infection and replication in 293 cells. In the present study, it was discovered that over-expression of human ADI1 in 293 cells (293-ADI1 cells) also supported HCV infection and replication. Using serum-derived HCV as an infectious source, enhanced cell uptake of HCV to a Northern blot detectable level was found in 293 cells over-expressing both CD81 and ADI1 (293-ADI1-CD81 cells). The enhanced cell entry was confirmed by the use of the vesicular stomatitis virus-based HCV pseudotype particles. However, transfection of HCV replicon RNA by electroporation into naive 293 and 293-ADI1 cells revealed no difference in replication efficiency. Using the infectious J6/JFH chimera as an infectious source, the infectivity was compared between 293-ADI1-CD81 and Huh-7.5 cells. More infection foci were formed in the 293-ADI1-CD81 cells in the first round of infection. In conclusion, human ADI1 over-expression in 293 cells enhances cell entry but not replication of HCV. 293-ADI1-CD81 cells are permissive for serum-derived HCV infection.
机译:人aci-还原酮双加氧酶1(ADI1)是Cupin超家族的成员。它结合并抑制1型膜基质金属蛋白酶的活性,该酶是一种已知与紧密连接蛋白claudin-1相互作用的蛋白。以前,发现一种由ADI1氨基酸64-179组成的变体蛋白,称为淹没诱导蛋白样因子(Sip-L),可支持丙型肝炎病毒(HCV)感染和在293细胞中复制。在本研究中,发现人ADI1在293细胞(293-ADI1细胞)中的过表达也支持HCV感染和复制。使用血清来源的HCV作为感染源,在过量表达CD81和ADI1的293细胞(293-ADI1-CD81细胞)中发现HCV的细胞摄取增加至Northern blot检测水平。通过使用基于水疱性口炎病毒的HCV假型颗粒,证实了细胞进入的增强。但是,通过电穿孔将HCV复制子RNA转染到原始293和293-ADI1细胞中,发现复制效率没有差异。使用传染性J6 / JFH嵌合体作为传染源,比较了293-ADI1-CD81和Huh-7.5细胞的传染性。在第一轮感染中,更多的感染灶在293-ADI1-CD81细胞中形成。总之,人ADI1在293细胞中的过度表达可增强细胞进入能力,但不会增强HCV的复制。 293-ADI1-CD81细胞可用于血清来源的HCV感染。

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