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传染性非细胞病变型HIV-2的env蛋白在合胞体形成方面存在缺陷。

The env protein of an infectious noncytopathic HIV-2 is deficient in syncytium formation.

作者信息

Mulligan M J, Kumar P, Hui H X, Owens R J, Ritter G D, Hahn B H, Compans R W

机构信息

Department of Medicine, University of Alabama, Birmingham 35294.

出版信息

AIDS Res Hum Retroviruses. 1990 Jun;6(6):707-20. doi: 10.1089/aid.1990.6.707.

Abstract

A recent isolate of human immunodeficiency virus type 2 (HIV-2) designated HIV-2ST is deficient in its ability to cause the typical cytopathic effects of HIV infection. The pathogenic potential of HIV-2 in inducing human disease may be less than that of HIV-1, and it is of particular interest to establish the basis for the reduced cytopathogenicity of this isolate in vitro. Utilizing recombinant vaccinia viruses (rVV) carrying the envelope genes (env) of HIV-2ST or those of fully cytopathic HIV-1 or HIV-2 isolates, we have investigated envelope glycoprotein expression, processing, transport, and biological function. Radioimmunoprecipitation and polyacrylamide gel electrophoresis (RIP-PAGE) of rVV-infected cell lysates indicated that the proteins expressed by each recombinant were synthesized, processed, and recognized by specific antisera. Immunofluorescence studies showed that the recombinant env gene products of HIV-2ST and HIV-2ROD reach the cell surface and are retained there in similar amounts. Whereas cells expressing the HIV-1 or HIV-2ROD env gene products were found to undergo fusion with uninfected CD4+ cells, no syncytium formation was observed with three CD4+ cell lines exposed to the cells expressing the envelope glycoproteins of HIV-2ST on their surfaces; one CD4+ lymphoid cell line (SupT1) exhibited few very small syncytia in the presence of recombinant HIV-2ST envelope glycoproteins. The failure of the HIV-2ST envelope glycoprotein to induce cell fusion was not the result of an inhibition by cell-associated CD4, since fusion was also not observed when rVVST-infected CD4- cells were cocultured with CD4+ cells. Thus, the HIV-2ST envelope protein itself is defective in its ability to induce cell fusion. Furthermore, the expression, processing, transport, and surface stability of env products of HIV-2ST are unlikely to be responsible for its attenuation, suggesting that the molecular interactions between its env products and target cell membranes are significantly altered.

摘要

最近分离出的一株2型人类免疫缺陷病毒(HIV-2),命名为HIV-2ST,在引发HIV感染典型细胞病变效应方面能力不足。HIV-2诱发人类疾病的致病潜力可能低于HIV-1,因此确定该分离株在体外细胞病变性降低的基础具有特别重要的意义。利用携带HIV-2ST包膜基因(env)或具有完全细胞病变性的HIV-1或HIV-2分离株包膜基因的重组痘苗病毒(rVV),我们研究了包膜糖蛋白的表达、加工、运输及生物学功能。对rVV感染的细胞裂解物进行放射免疫沉淀和聚丙烯酰胺凝胶电泳(RIP-PAGE)分析表明,每种重组体表达的蛋白质均能被合成、加工,并被特异性抗血清识别。免疫荧光研究显示,HIV-2ST和HIV-2ROD的重组env基因产物到达细胞表面,并以相似的量保留在那里。虽然发现表达HIV-1或HIV-2ROD env基因产物的细胞与未感染的CD4+细胞发生融合,但将三种CD4+细胞系暴露于表面表达HIV-2ST包膜糖蛋白的细胞时,未观察到合胞体形成;在存在重组HIV-2ST包膜糖蛋白的情况下,一种CD4+淋巴细胞系(SupT1)出现了少量非常小的合胞体。HIV-2ST包膜糖蛋白未能诱导细胞融合并非细胞相关CD4抑制的结果,因为当rVVST感染的CD4-细胞与CD4+细胞共培养时也未观察到融合。因此,HIV-2ST包膜蛋白本身诱导细胞融合的能力存在缺陷。此外,HIV-2ST的env产物的表达、加工、运输及表面稳定性不太可能是其减毒的原因,这表明其env产物与靶细胞膜之间的分子相互作用发生了显著改变。

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