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碱基、戊糖和磷酸二酯主链结构对大肠杆菌DNA光解酶结合和修复嘧啶二聚体的影响。

Effect of base, pentose, and phosphodiester backbone structures on binding and repair of pyrimidine dimers by Escherichia coli DNA photolyase.

作者信息

Kim S T, Sancar A

机构信息

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

出版信息

Biochemistry. 1991 Sep 3;30(35):8623-30. doi: 10.1021/bi00099a019.

Abstract

Photolyases reverse the effects of UV light on cells by converting cyclobutane dipyrimidine photoproducts (pyrimidine dimers, Pyr mean value of Pyr) into pyrimidine monomers in a light-dependent reaction. Previous work has suggested that, based on substrate preference, there are two classes of photolyase: DNA photolyase as exemplified by the Escherichia coli enzyme, and RNA photolyases found in plants such as Nicotiana tabacum and Phaseolus vulgaris. In experiments aimed at identifying substrate determinants, including the pentose ring, for binding and catalysis by E. coli DNA photolyase we tested several Pyr mean value of Pyr. We found that the enzyme has relative affinities for photodimers of T mean value of T greater than or equal to U mean value of T greater than U mean value of U much greater than C mean value of C and that the E-FADH2 form of the enzyme repairs these dimers at 366 nm with absolute quantum yields of 0.9 (T mean value of T), 0.8 (U mean value of T), 0.6 (U mean value of U), and 0.05 (C mean value of C). The enzyme also repairs an isolated thymine dimer and the synthetic substrate, 1,1'-trimethylene-bis (thymine) cyclobutane dimer. Unexpectedly, we found that this enzyme, previously thought to be specific for DNA, repairs uracil cyclobutane dimers in poly(rU). The affinity of photolyase for a uracil dimer in RNA is about 10(4)-fold lower than that for a U mean value of U in DNA; however, once bound, the enzyme repairs the photodimer with the same quantum yield whether the dimer is in ribonucleoside or deoxyribonucleoside form.

摘要

光解酶通过在光依赖反应中将环丁烷二嘧啶光产物(嘧啶二聚体,Pyr的平均值)转化为嘧啶单体,逆转紫外线对细胞的影响。先前的研究表明,根据底物偏好,光解酶有两类:以大肠杆菌酶为例的DNA光解酶,以及在烟草和菜豆等植物中发现的RNA光解酶。在旨在确定包括戊糖环在内的底物决定因素对大肠杆菌DNA光解酶结合和催化作用的实验中,我们测试了几种Pyr的平均值。我们发现,该酶对T的平均值的光二聚体的相对亲和力大于或等于U的平均值的T大于U的平均值的U远大于C的平均值的C,并且该酶的E-FADH2形式在366nm处修复这些二聚体,绝对量子产率分别为0.9(T的平均值)、0.8(U的平均值的T)、0.6(U的平均值的U)和0.05(C的平均值的C)。该酶还能修复分离的胸腺嘧啶二聚体和合成底物1,1'-三亚甲基-双(胸腺嘧啶)环丁烷二聚体。出乎意料的是,我们发现这种以前被认为对DNA具有特异性的酶能修复聚(rU)中的尿嘧啶环丁烷二聚体。光解酶对RNA中尿嘧啶二聚体的亲和力比对DNA中U的平均值的亲和力低约10^4倍;然而,一旦结合,无论二聚体是核糖核苷形式还是脱氧核糖核苷形式,该酶都以相同的量子产率修复光二聚体。

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