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利用DNA光解酶进行的时间分辨电子顺磁共振研究:激发态的FADH0从色氨酸-306提取一个电子以生成FADH-,即辅因子的催化活性形式。

Time-resolved EPR studies with DNA photolyase: excited-state FADH0 abstracts an electron from Trp-306 to generate FADH-, the catalytically active form of the cofactor.

作者信息

Kim S T, Sancar A, Essenmacher C, Babcock G T

机构信息

Department of Biochemistry and Biophysics, University of North Carolina School of Medicine, Chapel Hill 27599.

出版信息

Proc Natl Acad Sci U S A. 1993 Sep 1;90(17):8023-7. doi: 10.1073/pnas.90.17.8023.

Abstract

Photolyase repairs UV-induced cyclobutane-pyrimidine dimers in DNA by photoinduced electron transfer. The enzyme isolated from Escherichia coli contains 5,10-methenyltetrahydrofolate, which functions as the light-harvesting chromophore, and fully reduced flavin adenine dinucleotide (FAD), which functions as the redox catalyst. During enzyme preparation, the flavin is oxidized to FADH0, which is catalytically inert. Illumination of the enzyme with 300- to 600-nm light converts the flavin to the fully reduced form in a reaction that involves photooxidation of an amino acid in the apoenzyme. The results of earlier optical studies had indicated that the redox-active amino acid in this photoactivation process was tryptophan. We have now used time-resolved electron paramagnetic resonance (EPR) spectroscopy to investigate the photoactivation reaction. Excitation of the flavin-radical-containing inactive enzyme produces a spin-polarized radical that we identify by 2H and 15N labeling as originating from a tryptophan residue, confirming the inferences from the optical work. These results and Trp-->Phe replacement by site-directed mutagenesis reveal that flavin radical photoreduction is achieved by electron abstraction from Trp-306 by the excited-state FADH0. Analysis of the hyperfine couplings and spin density distribution deduced from the isotopic-labeling results shows that the product of the light-driven redox chemistry is the Trp-306 cation radical. The results strongly suggest that the active form of photolyase contains FADH- and not FADH2.

摘要

光解酶通过光诱导电子转移修复DNA中紫外线诱导的环丁烷嘧啶二聚体。从大肠杆菌中分离出的这种酶含有作为光捕获发色团的5,10-亚甲基四氢叶酸,以及作为氧化还原催化剂的完全还原型黄素腺嘌呤二核苷酸(FAD)。在酶的制备过程中,黄素被氧化为FADH0,而FADH0是没有催化活性的。用300至600纳米的光照射该酶,会在一个涉及脱辅基酶中氨基酸光氧化的反应中将黄素转化为完全还原形式。早期光学研究的结果表明,在这个光激活过程中具有氧化还原活性的氨基酸是色氨酸。我们现在使用时间分辨电子顺磁共振(EPR)光谱来研究光激活反应。对含有黄素自由基的无活性酶进行激发会产生一个自旋极化自由基,我们通过2H和15N标记确定其源自一个色氨酸残基,这证实了光学研究得出的推断。这些结果以及通过定点诱变将色氨酸替换为苯丙氨酸的实验表明,黄素自由基的光还原是通过激发态FADH0从色氨酸-306夺取电子来实现的。对由同位素标记结果推导得出的超精细偶合和自旋密度分布的分析表明,光驱动氧化还原化学反应的产物是色氨酸-306阳离子自由基。这些结果有力地表明,光解酶的活性形式含有FADH-而非FADH2。

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