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培养的人滋养层细胞对1型人类免疫缺陷病毒感染的易感性。

Susceptibility of cultured human trophoblasts to infection with human immunodeficiency virus type 1.

作者信息

Zachar V, Nørskov-Lauritsen N, Juhl C, Spire B, Chermann J C, Ebbesen P

机构信息

Danish Cancer Society, Department of Virus and Cancer, Aarhus C.

出版信息

J Gen Virol. 1991 Jun;72 ( Pt 6):1253-60. doi: 10.1099/0022-1317-72-6-1253.

DOI:10.1099/0022-1317-72-6-1253
PMID:2045791
Abstract

Primary cultures of essentially pure human term trophoblasts were studied to determine their ability to support the expression of complete proviral clones of human immunodeficiency virus (HIV) and their permissiveness to this virus. Transient expression of molecular clones derived from two biologically distinct strains, BRU and NDK, resulted in the release of comparable amounts of infectious virions, which were rescued by cocultivation with permissive CEM-SS cells. Trophoblasts were inoculated with three HIV-1 isolates, RF, 3B and NDK, which differ in their cytopathogenicity on T lymphoblastoid cells. Infection of cells by all three strains was demonstrated by the presence of virus-specific proteins in the trophoblasts and the detection of virus gag gene-related DNA sequences by the polymerase chain reaction (PCR), but cells were more susceptible to infection with the RF and NDK strains than with the 3B strain. The virus was readily transmitted to the CEM-SS cells with simultaneous formation of syncytia between the two cell types. Flow cytometry and direct radioimmunoassay revealed no trace of the CD4 receptor on the surface of the cultured trophoblasts and CD4 mRNA could not be detected by Northern blot hybridization, although a minimal amount of CD4-associated mRNA was detected by PCR. Our data suggest that infection of trophoblasts occurs independently of the pathway mediated by CD4.

摘要

对基本纯化的人足月滋养层细胞的原代培养物进行了研究,以确定它们支持人类免疫缺陷病毒(HIV)完整前病毒克隆表达的能力及其对该病毒的易感性。来自两种生物学上不同毒株BRU和NDK的分子克隆的瞬时表达导致释放出相当数量的感染性病毒粒子,这些病毒粒子通过与允许性的CEM-SS细胞共培养而被拯救出来。用三种HIV-1分离株RF、3B和NDK接种滋养层细胞,这三种分离株在T淋巴母细胞上的细胞致病性有所不同。通过滋养层细胞中存在病毒特异性蛋白以及通过聚合酶链反应(PCR)检测病毒gag基因相关DNA序列,证明了所有三种毒株均能感染细胞,但细胞对RF和NDK毒株的感染比3B毒株更敏感。病毒很容易传播到CEM-SS细胞,同时在两种细胞类型之间形成多核巨细胞。流式细胞术和直接放射免疫测定显示,培养的滋养层细胞表面没有CD4受体的痕迹,Northern印迹杂交检测不到CD4 mRNA,尽管通过PCR检测到少量与CD4相关的mRNA。我们的数据表明,滋养层细胞的感染独立于由CD4介导的途径发生。

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Clin Exp Immunol. 2001 Sep;125(3):455-64. doi: 10.1046/j.1365-2249.2001.01629.x.
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