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噬菌体T4 uvsY重组蛋白氨基末端片段的特性分析

Characterization of an amino-terminal fragment of the bacteriophage T4 uvsY recombination protein.

作者信息

Yassa D S, Chou K M, Morrical S W

机构信息

Department of Biochemistry, University of Vermont College of Medicine, Burlington 05405, USA.

出版信息

Biochimie. 1997 May;79(5):275-85. doi: 10.1016/s0300-9084(97)83515-8.

DOI:10.1016/s0300-9084(97)83515-8
PMID:9258436
Abstract

The uvsY protein plays essential roles in homologous genetic recombination processes in the bacteriophage T4. In vitro, uvsY promotes the formation of presynaptic filaments containing stoichiometric amounts of the T4 uvsX recombinase bound to single-stranded DNA. uvsY protein has intrinsic binding activities towards ssDNA, uvsX, and gp32, the T4-encoded SSB, however, it has not been directly determined which of these activities are essential for uvsY's role in presynapsis. We have therefore sought to generate altered forms of uvsY deficient in uvsX- and/or gp32-binding, in order to assess whether these specific protein-protein interactions are essential for uvsY recombination functions. Limited chymotrypsinolysis of the 16 kDa uvsY protein generates two major fragments: an 11.5 kDa fragment containing the N-terminus of uvsY, and a 4.5 kDa C-terminal fragment. We have expressed and purified the large fragment as a fusion protein containing the N-terminal 101 amino acids of uvsY. We show that this truncated uvsY species, which we call uvsYNT, retains ssDNA-binding activity, but is devoid of both uvsX- and gp32-binding activities. Like native uvsY, uvsYNT stimulates the ssDNA-dependent ATPase activity of the uvsX protein, however, the synergistic effects observed between uvsY, uvsX, and gp32 are not observed with uvsYNT. In addition, uvsYNT weakly stimulates uvsX-catalyzed DNA strand exchange reactions. The latter result is surprising since it suggests that specific interactions with uvsX and/or gp32 are not absolutely essential for uvsY recombination functions. Taken together, the data are consistent with a model in which uvsY-ssDNA interactions alone are capable of promoting the assembly of functional uvsX-ssDNA complexes, while uvsY-protein interactions stabilize uvsX-ssDNA complexes.

摘要

uvsY蛋白在噬菌体T4的同源基因重组过程中发挥着重要作用。在体外,uvsY促进了包含化学计量的与单链DNA结合的T4 uvsX重组酶的突触前细丝的形成。uvsY蛋白对单链DNA、uvsX和gp32(T4编码的单链结合蛋白)具有内在结合活性,然而,尚未直接确定这些活性中哪一种对uvsY在突触前的作用至关重要。因此,我们试图生成缺乏uvsX和/或gp32结合的uvsY变体形式,以评估这些特定的蛋白质-蛋白质相互作用对于uvsY重组功能是否必不可少。对16 kDa的uvsY蛋白进行有限的胰凝乳蛋白酶水解产生两个主要片段:一个包含uvsY N端的11.5 kDa片段和一个4.5 kDa的C端片段。我们已将大片段表达并纯化为包含uvsY N端101个氨基酸的融合蛋白。我们表明,这种截短的uvsY物种,我们称之为uvsYNT,保留了单链DNA结合活性,但缺乏uvsX和gp32结合活性。与天然uvsY一样,uvsYNT刺激uvsX蛋白的单链DNA依赖性ATP酶活性,然而,在uvsYNT中未观察到uvsY、uvsX和gp32之间观察到的协同效应。此外,uvsYNT微弱地刺激uvsX催化的DNA链交换反应。后一个结果令人惊讶,因为它表明与uvsX和/或gp32的特定相互作用对于uvsY重组功能并非绝对必要。综上所述,这些数据与一个模型一致,在该模型中,单独的uvsY-单链DNA相互作用能够促进功能性uvsX-单链DNA复合物的组装,而uvsY-蛋白质相互作用稳定uvsX-单链DNA复合物。

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