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嗜热四膜虫端粒末端结合蛋白复合物中的核苷酸重排与单链DNA识别

Nucleotide shuffling and ssDNA recognition in Oxytricha nova telomere end-binding protein complexes.

作者信息

Theobald Douglas L, Schultz Steve C

机构信息

Department of Chemistry and Biochemistry, University of Colorado at Boulder, Boulder, CO 80309-0215, USA.

出版信息

EMBO J. 2003 Aug 15;22(16):4314-24. doi: 10.1093/emboj/cdg415.

Abstract

Sequence-specific protein recognition of single-stranded nucleic acids is critical for many fundamental cellular processes, such as DNA replication, DNA repair, transcription, translation, recombination, apoptosis and telomere maintenance. To explore the mechanisms of sequence-specific ssDNA recognition, we determined the crystal structures of 10 different non-cognate ssDNAs complexed with the Oxytricha nova telomere end-binding protein (OnTEBP) and evaluated their corresponding binding affinities (PDB ID codes 1PH1-1PH9 and 1PHJ). The thermodynamic and structural effects of these sequence perturbations could not have been predicted based solely upon the cognate structure. OnTEBP accommodates non-cognate nucleotides by both subtle adjustments and surprisingly large structural rearrangements in the ssDNA. In two complexes containing ssDNA intermediates that occur during telomere extension by telomerase, entire nucleotides are expelled from the complex. Concurrently, the sequence register of the ssDNA shifts to re-establish a more cognate-like pattern. This phenomenon, termed nucleotide shuffling, may be of general importance in protein recognition of single-stranded nucleic acids. This set of structural and thermodynamic data highlights a fundamental difference between protein recognition of ssDNA versus dsDNA.

摘要

单链核酸的序列特异性蛋白质识别对于许多基本细胞过程至关重要,如DNA复制、DNA修复、转录、翻译、重组、细胞凋亡和端粒维持。为了探索序列特异性单链DNA识别的机制,我们确定了与新大草履虫端粒末端结合蛋白(OnTEBP)复合的10种不同非同源单链DNA的晶体结构,并评估了它们相应的结合亲和力(PDB ID编码1PH1 - 1PH9和1PHJ)。仅基于同源结构无法预测这些序列扰动的热力学和结构效应。OnTEBP通过单链DNA中的细微调整和惊人的大结构重排来容纳非同源核苷酸。在两种含有端粒酶延伸端粒过程中出现的单链DNA中间体的复合物中,整个核苷酸从复合物中排出。同时,单链DNA的序列对齐发生变化,以重新建立更类似同源的模式。这种现象称为核苷酸重排,可能在单链核酸的蛋白质识别中具有普遍重要性。这组结构和热力学数据突出了蛋白质对单链DNA与双链DNA识别之间的根本差异。

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