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猫免疫缺陷病毒逆转录酶:66千道尔顿和51千道尔顿亚基的表达、功能特性及重组

Feline immunodeficiency virus reverse transcriptase: expression, functional characterization, and reconstitution of the 66- and 51-kilodalton subunits.

作者信息

Amacker M, Hottiger M, Hübscher U

机构信息

Institute of Veterinary Biochemistry, University of Zürich-Irchel, Switzerland.

出版信息

J Virol. 1995 Oct;69(10):6273-9. doi: 10.1128/JVI.69.10.6273-6279.1995.

Abstract

The two subunits of the feline immunodeficiency virus (FIV) reverse transcriptase (RT) were cloned and functionally expressed in Escherichia coli. The recombinant proteins are enzymatically active as homodimers (p66 and p51) as well as a heterodimer p66/p51. The biochemical properties of the FIV RT are very similar to those of the counterpart of the human immunodeficiency virus type 1 in being an RNA-dependent and DNA-dependent DNA polymerase. When a double-stranded DNA containing a small gap of 26 nucleotides was tested, we found a new activity of the FIV RT p66/p51 heterodimer--the cat viral enzyme could perform strand displacement DNA synthesis of approximately 300 bases. The FIV RT homodimer p66 alone could carry out limited strand displacement DNA synthesis, but this activity was stimulated by the p51 subunit at a molar ratio of one molecule of p66 to five molecules of p51. On the other hand, the homodimeric p51 itself was unable to fill a small gap of 26 nucleotides in a double-stranded DNA substrate and was not active by itself in strand displacement DNA synthesis. These data are in agreement with an earlier finding of strand displacement DNA synthesis by human immunodeficiency virus type 1 RT (M. Hottiger, V.N. Podust, R.L. Thimmig, C.S. McHenry, and U. Hübscher. J. Biol. Chem. 269:986-991, 1994). Our data therefore suggest a general and important function of lentiviral p51 subunits in strand displacement DNA synthesis which appears to be required in later stages of the lentiviral replication cycle, when DNA-dependent DNA synthesis occurs on double-stranded DNA.

摘要

猫免疫缺陷病毒(FIV)逆转录酶(RT)的两个亚基在大肠杆菌中被克隆并实现了功能表达。重组蛋白作为同型二聚体(p66和p51)以及异型二聚体p66/p51具有酶活性。FIV RT的生化特性与人类免疫缺陷病毒1型的对应物非常相似,都是依赖RNA和依赖DNA的DNA聚合酶。当测试含有26个核苷酸小缺口的双链DNA时,我们发现FIV RT p66/p51异型二聚体有一项新活性——这种猫病毒酶能够进行约300个碱基的链置换DNA合成。单独的FIV RT同型二聚体p66能够进行有限的链置换DNA合成,但该活性受到p51亚基的刺激,二者的摩尔比为一个p66分子比五个p51分子。另一方面,同型二聚体p51本身无法填补双链DNA底物中26个核苷酸的小缺口,自身在链置换DNA合成中也无活性。这些数据与早期关于人类免疫缺陷病毒1型RT进行链置换DNA合成的发现一致(M. Hottiger、V.N. Podust、R.L. Thimmig、C.S. McHenry和U. Hübscher。《生物化学杂志》269:986 - 991,1994)。因此,我们的数据表明慢病毒p51亚基在链置换DNA合成中具有普遍且重要的功能,这似乎是慢病毒复制周期后期所必需的,此时依赖DNA的DNA合成发生在双链DNA上。

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