首页> 外文期刊>Nucleic Acids Research >Substrate specificity of ultraviolet DNA endonuclease (UVDE/Uve1p) from Schizosaccharomyces pombe.
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Substrate specificity of ultraviolet DNA endonuclease (UVDE/Uve1p) from Schizosaccharomyces pombe.

机译:粟酒裂殖酵母中紫外线DNA核酸内切酶(UVDE / Uve1p)的底物特异性。

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摘要

Schizosaccharomyces pombe ultraviolet DNA endonuclease (UVDE or Uve1p) has been shown to cleave 5' to UV light-induced cyclobutane pyrimidine dimers (CPDs) and pyrimidine-pyrimidone (6-4) photoproducts (6-4PP). This endonuclease is believed to function in the initial step in an alternative excision repair pathway for the removal of DNA damage caused by exposure to UV light. An active truncated form of this protein, Delta228-Uve1p, has been successfully overexpressed, affinity purified and partially characterized. In the present study we present data from a detailed substrate specificity trial. We have determined that the substrate range of Uve1p is much greater than was originally believed. We demonstrate that this DNA damage repair protein is capable of recognizing an array of UV-induced DNA photoproducts (cis-syn-, trans-syn I- and trans-syn II CPDs, 6-4PP and Dewar isomers) that cause varying degrees of distortion in a duplex DNA molecule. We also demonstrate that Uve1p recognizes non-UV-induced DNA damage, such as platinum-DNA GG diadducts, uracil, dihydrouracil and abasic sites. This is the first time that a single DNA repair endonuclease with the ability to recognize such a diverse range of lesions has been described. This study suggests that Uve1p and the alternative excision repair pathway may participate broadly in the repair of DNA damage.
机译:粟酒裂殖酵母紫外线DNA核酸内切酶(UVDE或Uve1p)已显示可将5'裂解为紫外线诱导的环丁烷嘧啶二聚体(CPD)和嘧啶-嘧啶(6-4)光产物(6-4PP)。据信该核酸内切酶在替代切除修复途径的初始步骤中起作用,以消除由暴露于紫外线引起的DNA损伤。该蛋白的活性截短形式Delta228-Uve1p已成功过表达,亲和纯化并部分表征。在本研究中,我们提供了来自详细的底物特异性试验的数据。我们已经确定,Uve1p的底物范围比最初认为的要大得多。我们证明,这种DNA损伤修复蛋白能够识别引起不同程度的UV诱导的DNA光产物(顺式,顺式,反式I和反式II CPD,6-4PP和杜瓦异构体)的阵列。双链DNA分子中的畸变。我们还证明了Uve1p识别非紫外线诱导的DNA损伤,例如铂DNA GG二加合物,尿嘧啶,二氢尿嘧啶和无碱基位点。这是首次描述了具有识别这种不同范围病变能力的单个DNA修复核酸内切酶。这项研究表明Uve1p和替代切除修复途径可能广泛参与DNA损伤的修复。

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