Functional Characterization of Zinc-Finger Motif in Redox Regulation of RPA−ssDNA Interaction

锌指 半胱氨酸 化学 锌指核酸酶 DTNB公司 DNA 无名指区 DNA结合蛋白 氧化还原 突变体 LIM域 复制蛋白A 生物化学 转录因子 谷胱甘肽 无机化学 有机化学 基因
作者
Jinsam You,Mu Wang,Suk‐Hee Lee
出处
期刊:Biochemistry [American Chemical Society]
卷期号:39 (42): 12953-12958 被引量:27
标识
DOI:10.1021/bi001206f
摘要

The 70-kDa subunit of eukaryotic replication protein A (RPA) contains a conserved four cysteine-type zinc-finger motif that has been implicated in regulation of DNA replication and repair. Unlike other zinc-finger proteins, RPA zinc-finger motif is not a DNA-binding component, and deletion of the zinc-finger had very little effect on its ssDNA binding activity. Recently, we described a novel function for the zinc-finger motif in regulation of RPA's ssDNA binding activity through reduction−oxidation (redox). In this study, we carried out a detailed analysis of wild-type RPA and zinc-finger mutants in redox regulation of their ssDNA binding activity. Any mutation at a zinc-finger cysteine abolished its redox role in regulation of RPA−ssDNA interaction, suggesting that all four zinc-finger cysteines are required for redox regulation. Reactivity of cysteine residues to 5,5'-dithiobis(2-nitrobenzoic acid) (DTNB) indicated that wild-type RPA contained 8.2 reactive thiols/molecule including all four cysteines in the zinc-finger motif. Zinc-finger cysteines slowly reacted to DTNB as compared to others. Zn(II) was not only essential but also uniquely qualified for redox regulation of RPA−ssDNA interaction, suggesting that Zn(II)−cysteine coordination is crucial for the zinc-finger function. Redox status significantly affected initial interaction of RPA with ssDNA but had no effect after RPA formed a stable complex with DNA. Together, our results suggest that the zinc-finger motif mediates the transition of RPA−ssDNA interaction to a stable RPA−ssDNA complex in a redox-dependent manner.
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