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环丁烷嘧啶二聚体光解酶与隐色体 DASH 及其底物 DNA 复合物的光谱和生物物理化学研究综述。

A Review of Spectroscopic and Biophysical-Chemical Studies of the Complex of Cyclobutane Pyrimidine Dimer Photolyase and Cryptochrome DASH with Substrate DNA.

机构信息

Department of Chemistry and Biochemistry, Montclair State University, Montclair, NJ.

出版信息

Photochem Photobiol. 2017 Jan;93(1):26-36. doi: 10.1111/php.12678. Epub 2017 Jan 20.

Abstract

Cyclobutane pyrimidine dimer (CPD) photolyase (PL) is a structure-specific DNA repair enzyme that uses blue light to repair CPD on DNA. Cryptochrome (CRY) DASH enzymes use blue light for the repair of CPD lesions on single-stranded (ss) DNA, although some may also repair these lesions on double-stranded (ds) DNA. In addition, CRY DASH may be involved in blue light signaling, similar to cryptochromes. The focus of this review is on spectroscopic and biophysical-chemical experiments of the enzyme-substrate complex that have contributed to a more detailed understanding of all the aspects of the CPD repair mechanism of CPD photolyase and CRY DASH. This will be performed in the backdrop of the available X-ray crystal structures of these enzymes bound to a CPD-like lesion. These structures helped to confirm conclusions that were drawn earlier from spectroscopic and biophysical-chemical experiments, and they have a critical function as a framework to design new experiments and to interpret new experimental data. This review will show the important synergy between X-ray crystallography and spectroscopic/biophysical-chemical investigations that is essential to obtain a sufficiently detailed picture of the overall mechanism of CPD photolyases and CRY DASH proteins.

摘要

环丁烷嘧啶二聚体 (CPD) 光解酶 (PL) 是一种结构特异性的 DNA 修复酶,它利用蓝光修复 DNA 上的 CPD。隐花色素 (CRY) DASH 酶利用蓝光修复单链 (ss) DNA 上的 CPD 损伤,但有些酶也可能修复双链 (ds) DNA 上的这些损伤。此外,CRY DASH 可能参与蓝光信号转导,类似于隐花色素。本综述的重点是关于酶-底物复合物的光谱和生物物理化学实验,这些实验有助于更详细地了解 CPD 光解酶和 CRY DASH 的 CPD 修复机制的所有方面。这将在这些酶与 CPD 类似损伤结合的现有 X 射线晶体结构的背景下进行。这些结构有助于证实先前从光谱和生物物理化学实验中得出的结论,并作为设计新实验和解释新实验数据的关键框架发挥作用。本综述将展示 X 射线晶体学和光谱/生物物理化学研究之间的重要协同作用,这对于获得 CPD 光解酶和 CRY DASH 蛋白整体机制的足够详细的图像至关重要。

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