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与脱氧核糖核酸酶I形成的带切口的DNA八核苷酸复合物的结构精修至2埃。

Structure refined to 2A of a nicked DNA octanucleotide complex with DNase I.

作者信息

Suck D, Lahm A, Oefner C

机构信息

European Molecular Biology Laboratory, Biological Structures Division, Heidelberg, FRG.

出版信息

Nature. 1988 Mar 31;332(6163):464-8. doi: 10.1038/332464a0.

DOI:10.1038/332464a0
PMID:3352748
Abstract

The cutting rates of bovine pancreatic deoxyribonuclease I (DNase I) vary along a given DNA sequence, indicating that the enzyme recognizes sequence-dependent structural variations of the DNA double-helix. In an attempt to define the helical parameters determining this sequence-dependence, we have co-crystallized a complex of DNase I with a self-complementary octanucleotide and refined the crystal structure at 2 A resolution. This structure confirms the basic features of an early model, namely that an exposed loop of DNase I binds in the minor groove of B-type DNA and that interactions do occur with the backbone of both strands. Nicked octamer duplexes that have lost a dinucleotide from the 3'-end of one strand are hydrogen-bonded across a two-fold axis in the crystal to form a quasi-continuous double helix of 14 base pairs. The DNA 14-mer has a B-type conformation and shows substantial distortion of both local and overall helix parameters, induced mainly by the tight interaction of Y73 and R38 in the unusually wide minor groove. Directly coupled to the widening of the groove by approximately 3A is a 21.5 degree bend of the DNA away from the bound enzyme towards the major groove, suggesting that both DNA stiffness and groove width are important in determining the sequence-dependence of the enzyme cutting rate. A second cut of the DNA which is induced by diffusion of Mn2+ into the co-crystals suggests that there are two active sites in DNase I separated by more than 15A.

摘要

牛胰腺脱氧核糖核酸酶I(DNase I)的切割速率沿给定的DNA序列变化,这表明该酶能识别DNA双螺旋的序列依赖性结构变异。为了确定决定这种序列依赖性的螺旋参数,我们使DNase I与一个自互补八聚体形成复合物并进行共结晶,然后以2埃的分辨率对晶体结构进行了精修。该结构证实了早期模型的基本特征,即DNase I的一个暴露环结合在B型DNA的小沟中,并且确实与两条链的主链发生相互作用。从一条链的3'端缺失了一个二核苷酸的带切口的八聚体双链体在晶体中跨二重轴形成氢键,从而形成一个14个碱基对的准连续双螺旋。这个14聚体DNA具有B型构象,并且局部和整体螺旋参数都出现了显著扭曲,这主要是由异常宽的小沟中Y73和R38的紧密相互作用引起的。与小沟宽度增加约3埃直接相关的是,DNA从结合的酶处向大沟方向弯曲了21.5度,这表明DNA的刚性和沟宽在决定酶切割速率的序列依赖性方面都很重要。由Mn2+扩散到共晶体中引发的DNA的第二次切割表明,DNase I中有两个活性位点,它们之间的距离超过15埃。

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