Insights into the RNA binding mechanism of human L1-ORF1p: a molecular dynamics study†

IF 3.743 Q2 Biochemistry, Genetics and Molecular Biology
Muthukumaran Rajagopalan, Sangeetha Balasubramanian and Amutha Ramaswamy
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引用次数: 3

Abstract

The recognition and binding of nucleic acids by ORF1p, an L1 retrotransposon protein, have not yet been clearly understood due to the lack of structural knowledge. The present study attempts to identify the probable single-stranded RNA binding pathway of trimeric ORF1p using computational methods like ligand mapping methodology combined with molecular dynamics simulations. Using the ligand mapping methodology, the possible RNA interacting sites on the surface of the trimeric ORF1p were identified. The crystal structure of the ORF1p timer and an RNA molecule of 29 nucleotide bases in length were used to generate the structure of the ORF1p complex based on information on predicted binding sites as well as the functional states of the CTD. The various complexes of ORF1p–RNA were generated using polyU, polyA and L1RNA sequences and were simulated for a period of 75 ns. The observed stable interaction pattern was used to propose the possible binding pathway. Based on the binding free energy for complex formation, both polyU and L1RNA complexes were identified as stable complexes, while the complex formed with polyA was the least stable one. Furthermore, the importance of the residues in the CC domain (Lys137 and Arg141), the RRM loop (Arg206, Arg210 and Arg211) and the CTD (Arg 261 and Arg262) of all three chains in stabilizing the wrapped RNA has been highlighted in this study. The presence of several electrostatic interactions including H-bond interactions increases the affinity towards RNA and hence plays a vital role in retaining the wrapped position of RNA around ORF1p. Altogether, this study presents one of the possible RNA binding pathways of ORF1p and clearly highlights the functional state of ORF1p visited during RNA binding.

Abstract Image

人L1-ORF1p RNA结合机制的分子动力学研究
ORF1p是一种L1逆转录转座子蛋白,由于缺乏结构知识,目前对其对核酸的识别和结合尚不清楚。本研究试图利用配体作图等计算方法结合分子动力学模拟,确定三聚体ORF1p可能的单链RNA结合途径。利用配体定位方法,鉴定了三聚体ORF1p表面可能的RNA相互作用位点。ORF1p定时器的晶体结构和一个长度为29个核苷酸碱基的RNA分子基于预测结合位点的信息以及CTD的功能状态生成ORF1p复合物的结构。利用polyU、polyA和L1RNA序列生成ORF1p-RNA的各种复合物,模拟时间为75 ns。利用观察到的稳定相互作用模式提出了可能的结合途径。根据络合物形成的结合自由能,polyU和L1RNA都是稳定的络合物,而polyA形成的络合物是最不稳定的络合物。此外,本研究还强调了CC结构域(Lys137和Arg141)、RRM环(Arg206、Arg210和Arg211)和CTD (Arg 261和Arg262)上的残基对稳定包裹RNA的重要性。包括氢键相互作用在内的几种静电相互作用的存在增加了对RNA的亲和力,因此在保持RNA在ORF1p周围的包裹位置方面起着至关重要的作用。总之,本研究提出了ORF1p可能的RNA结合途径之一,并清楚地强调了ORF1p在RNA结合过程中所访问的功能状态。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Molecular BioSystems
Molecular BioSystems 生物-生化与分子生物学
CiteScore
2.94
自引率
0.00%
发文量
0
审稿时长
2.6 months
期刊介绍: Molecular Omics publishes molecular level experimental and bioinformatics research in the -omics sciences, including genomics, proteomics, transcriptomics and metabolomics. We will also welcome multidisciplinary papers presenting studies combining different types of omics, or the interface of omics and other fields such as systems biology or chemical biology.
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