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对环孢素A耐药的1型人类免疫缺陷病毒突变体表明,Gag编码亲环素A的功能靶点。

Cyclosporine A-resistant human immunodeficiency virus type 1 mutants demonstrate that Gag encodes the functional target of cyclophilin A.

作者信息

Braaten D, Aberham C, Franke E K, Yin L, Phares W, Luban J

机构信息

Department of Microbiology, Columbia University College of Physicians and Surgeons, New York 10032, USA.

出版信息

J Virol. 1996 Aug;70(8):5170-6. doi: 10.1128/JVI.70.8.5170-5176.1996.

Abstract

The cellular peptidyl-prolyl isomerase cyclophilin A is incorporated into human immunodeficiency virus type 1 virions via contacts with the proline-rich domain of the Gag polyprotein. Cyclosporine A and nonimmunosuppressive analogs bind with high affinity to cyclophilin A, compete with Gag for binding to cyclophilin A, and prevent incorporation of cyclophilin A into virions; in parallel with the disruption of cyclophilin A incorporation into virions, there is a linear reduction in the initiation of reverse transcription after infection of a T cell. Passage of human immunodeficiency virus type 1 in the presence of the drug selects one of two mutations, either of which alters the proline-rich domain of Gag and is sufficient to confer drug resistance on the cloned wild-type provirus. Neither mutation alters Gag's cyclophilin A-binding properties in vitro, and cyclophilin A incorporation into drug-resistant virions is effectively disrupted by cyclosporine A, indicating that the drug-resistant mutants do not require virion-associated cyclophilin A to initiate infection. That Gag's functional dependence on cyclophilin A can be differentiated genetically from its ability to bind cyclophilin A is further demonstrated by the rescue of a mutation precluding cyclophilin A packaging by a mutation conferring cyclosporine A resistance. These experiments demonstrate that, in addition to its ability to package cyclophilin A into virions, gag encodes the functional target of cyclophilin A.

摘要

细胞内肽基脯氨酰异构酶亲环蛋白A通过与Gag多蛋白富含脯氨酸的结构域接触而被整合到人免疫缺陷病毒1型病毒粒子中。环孢素A和非免疫抑制类似物与亲环蛋白A高亲和力结合,与Gag竞争结合亲环蛋白A,并阻止亲环蛋白A整合到病毒粒子中;与亲环蛋白A整合到病毒粒子的破坏同时发生的是,T细胞感染后逆转录起始呈线性减少。在药物存在的情况下传代人免疫缺陷病毒1型会选择两种突变之一,这两种突变中的任何一种都会改变Gag的富含脯氨酸结构域,并且足以赋予克隆的野生型前病毒耐药性。这两种突变在体外均不改变Gag与亲环蛋白A的结合特性,环孢素A可有效破坏亲环蛋白A整合到耐药病毒粒子中,这表明耐药突变体在启动感染时不需要病毒粒子相关的亲环蛋白A。赋予环孢素A抗性的突变对排除亲环蛋白A包装的突变的挽救进一步证明,Gag对亲环蛋白A的功能依赖性与其结合亲环蛋白A的能力在遗传上是可区分的。这些实验表明,除了将亲环蛋白A包装到病毒粒子中的能力外,gag还编码亲环蛋白A的功能靶点。

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