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原子分辨率研究 S1 核酸酶复合物揭示了尽管存在多个晶格易位缺陷,但 RNA 与酶相互作用的细节。

Atomic resolution studies of S1 nuclease complexes reveal details of RNA interaction with the enzyme despite multiple lattice-translocation defects.

机构信息

Institute of Biotechnology, Czech Academy of Sciences, v.v.i., Průmyslová 595, 252 50 Vestec, Czech Republic.

Novozymes A/S, Biologiens Vej 2, DK-2880 Kgs Lyngby, Denmark.

出版信息

Acta Crystallogr D Struct Biol. 2022 Oct 1;78(Pt 10):1194-1209. doi: 10.1107/S2059798322008397. Epub 2022 Sep 27.

DOI:10.1107/S2059798322008397
PMID:36189740
Abstract

S1 nuclease from Aspergillus oryzae is a single-strand-specific nuclease from the S1/P1 family that is utilized in biochemistry and biotechnology. S1 nuclease is active on both RNA and DNA but with differing catalytic efficiencies. This study clarifies its catalytic properties using a thorough comparison of differences in the binding of RNA and DNA in the active site of S1 nuclease based on X-ray structures, including two newly solved complexes of S1 nuclease with the products of RNA cleavage at atomic resolution. Conclusions derived from this comparison are valid for the whole S1/P1 nuclease family. For proper model building and refinement, multiple lattice-translocation defects present in the measured diffraction data needed to be solved. Two different approaches were tested and compared. Correction of the measured intensities proved to be superior to the use of the dislocation model of asymmetric units with partial occupancy of individual chains. As the crystals suffered from multiple lattice translocations, equations for their correction were derived de novo. The presented approach to the correction of multiple lattice-translocation defects may help to solve similar problems in the field of protein X-ray crystallography.

摘要

米曲霉 S1 核酸酶是 S1/P1 家族中的一种单链特异性核酸酶,在生物化学和生物技术中被广泛应用。S1 核酸酶可作用于 RNA 和 DNA,但催化效率有所不同。本研究通过比较 S1 核酸酶活性中心 RNA 和 DNA 的结合差异,利用 X 射线结构(包括两个新解析的 S1 核酸酶与 RNA 切割产物的原子分辨率复合物),对其催化特性进行了全面解析。从该比较中得出的结论对整个 S1/P1 核酸酶家族均适用。为了进行适当的模型构建和精修,需要解决测量衍射数据中存在的多个晶格平移缺陷。我们测试并比较了两种不同的方法。结果表明,对测量强度进行校正优于使用部分占据单个链的不对称单元的位错模型。由于晶体存在多个晶格平移,因此推导出了针对它们的校正方程。该方法可能有助于解决蛋白质 X 射线晶体学领域的类似问题。

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1
Atomic resolution studies of S1 nuclease complexes reveal details of RNA interaction with the enzyme despite multiple lattice-translocation defects.原子分辨率研究 S1 核酸酶复合物揭示了尽管存在多个晶格易位缺陷,但 RNA 与酶相互作用的细节。
Acta Crystallogr D Struct Biol. 2022 Oct 1;78(Pt 10):1194-1209. doi: 10.1107/S2059798322008397. Epub 2022 Sep 27.
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Structural and Catalytic Properties of S1 Nuclease from Aspergillus oryzae Responsible for Substrate Recognition, Cleavage, Non-Specificity, and Inhibition.米曲霉S1核酸酶的结构与催化特性:底物识别、切割、非特异性及抑制作用
PLoS One. 2016 Dec 30;11(12):e0168832. doi: 10.1371/journal.pone.0168832. eCollection 2016.
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Amino acid sequence of nuclease S1 from Aspergillus oryzae.米曲霉核酸酶S1的氨基酸序列。
J Biochem. 1991 Jul;110(1):151-8. doi: 10.1093/oxfordjournals.jbchem.a123534.
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Immobilization of single-strand specific nuclease (S1 nuclease) from Aspergillus oryzae.米曲霉单链特异性核酸酶(S1核酸酶)的固定化。
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The plant s1-like nuclease family has evolved a highly diverse range of catalytic capabilities.植物 s1 样核酸酶家族进化出了高度多样化的催化能力。
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Specificity of the S1 nuclease from Aspergillus oryzae.米曲霉S1核酸酶的特异性
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S1 nuclease: immunoaffinity purification and evidence for the proximity of cysteine 25 to the substrate binding site.S1核酸酶:免疫亲和纯化及半胱氨酸25靠近底物结合位点的证据
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Recognition of single-stranded DNA by nuclease P1: high resolution crystal structures of complexes with substrate analogs.核酸酶P1对单链DNA的识别:与底物类似物复合物的高分辨率晶体结构
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S1 nuclease hydrolysis of single-stranded nucleic acids with partial double-stranded configuration.S1核酸酶对具有部分双链结构的单链核酸的水解作用。
Biochemistry. 1975 Sep 23;14(19):4221-6. doi: 10.1021/bi00690a011.

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