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利用傅里叶变换红外光谱法检测光解酶与底物结合时环丁烷嘧啶二聚体的独特α-螺旋重排。

Detection of distinct α-helical rearrangements of cyclobutane pyrimidine dimer photolyase upon substrate binding by Fourier transform infrared spectroscopy.

机构信息

Department of Frontier Materials, Nagoya Institute of Technology, Nagoya 466-8555, Japan.

出版信息

Biochemistry. 2013 Feb 12;52(6):1019-27. doi: 10.1021/bi3016179. Epub 2013 Jan 30.

DOI:10.1021/bi3016179
PMID:23331252
Abstract

Photolyases (PHRs) utilize near-ultraviolet (UV)-blue light to specifically repair the major photoproducts (PPs) of UV-induced damaged DNA. The cyclobutane pyrimidine dimer PHR (CPD-PHR) from Escherichia coli binds flavin adenine dinucleotide (FAD) as a cofactor and 5,10-methenyltetrahydrofolate as a light-harvesting pigment and specifically repairs CPD lesions. By comparison, a second photolyase known as (6-4) PHR, present in a range of higher organisms, uniquely repairs (6-4) PPs. To understand the repair mechanism and the substrate specificity that distinguish CPD-PHR from (6-4) PHR, we applied Fourier transform infrared (FTIR) spectroscopy to bacterial CPD-PHR in the presence or absence of a well-defined DNA substrate, as we have studied previously for vertebrate (6-4) PHR. PHRs show light-induced reduction of FAD, and photorepair by CPD-PHR involves the transfer of an electron from the photoexcited reduced FAD to the damaged DNA for cleaving the dimers to maintain the DNA's integrity. Here, we measured and analyzed difference FTIR spectra for the photoactivation and DNA photorepair processes of CPD-PHR. We identified light-dependent signals only in the presence of substrate. The signals, presumably arising from a protonated carboxylic acid or the DNA substrate, implicate conformational rearrangements of the protein and substrate during the repair process. Deuterium exchange FTIR measurements of CPD-PHR highlight potential differences in the photoactivation and photorepair mechanisms in comparison to those of (6-4) PHR. Although CPD-PHR and (6-4) PHR appear to exhibit similar overall structures, our studies indicate that distinct conformational rearrangements, especially in the α-helices, are initiated within these enzymes upon binding of their respective DNA substrates.

摘要

光解酶(PHR)利用近紫外(UV)-蓝光特异性地修复 UV 诱导的 DNA 损伤的主要光产物(PPs)。来自大肠杆菌的环丁烷嘧啶二聚体 PHR(CPD-PHR)结合黄素腺嘌呤二核苷酸(FAD)作为辅因子和 5,10-亚甲基四氢叶酸作为光捕获色素,特异性修复 CPD 损伤。相比之下,另一种存在于多种高等生物中的第二种光解酶,即(6-4)PHR,唯一修复(6-4)PPs。为了理解区分 CPD-PHR 和(6-4)PHR 的修复机制和底物特异性,我们应用傅里叶变换红外(FTIR)光谱学研究了细菌 CPD-PHR 存在或不存在明确定义的 DNA 底物的情况下,正如我们之前对脊椎动物(6-4)PHR 所做的那样。PHR 显示 FAD 的光诱导还原,并且 CPD-PHR 的光修复涉及将电子从光激发的还原 FAD 转移到受损的 DNA 上,以切割二聚体以维持 DNA 的完整性。在这里,我们测量并分析了 CPD-PHR 的光激活和 DNA 光修复过程的差 FTIR 光谱。我们仅在存在底物的情况下检测到依赖于光的信号。这些信号可能来自质子化的羧酸或 DNA 底物,表明在修复过程中蛋白质和底物的构象重排。与(6-4)PHR 相比,CPD-PHR 的氘交换 FTIR 测量突出了光激活和光修复机制中的潜在差异。尽管 CPD-PHR 和(6-4)PHR 似乎表现出相似的整体结构,但我们的研究表明,在这些酶结合各自的 DNA 底物时,会引发独特的构象重排,尤其是在α-螺旋中。

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引用本文的文献

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Structural role of two histidines in the (6-4) photolyase reaction.两个组氨酸在(6-4)光解酶反应中的结构作用。
Biophys Physicobiol. 2015 Dec 22;12:139-44. doi: 10.2142/biophysico.12.0_139. eCollection 2015.
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FTIR study of CPD photolyase with substrate in single strand DNA.
用单链DNA中的底物对CPD光裂合酶进行傅里叶变换红外光谱研究。
Biophysics (Nagoya-shi). 2015 Feb 13;11:39-45. doi: 10.2142/biophysics.11.39. eCollection 2015.