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一种具有新型单价阳离子介导折叠的 RNA 适体通过抑制长天然底物的结合来抑制溶菌酶的催化作用。

An RNA aptamer possessing a novel monovalent cation-mediated fold inhibits lysozyme catalysis by inhibiting the binding of long natural substrates.

出版信息

RNA. 2014 Apr;20(4):447-61. doi: 10.1261/rna.043034.113. Epub 2014 Feb 25.

DOI:10.1261/rna.043034.113
PMID:24570482
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3964907/
Abstract

RNA aptamers are being developed as inhibitors of macromolecular and cellular function, diagnostic tools, and potential therapeutics. Our understanding of the physical nature of this emerging class of nucleic acid-protein complexes is limited; few atomic resolution structures have been reported for aptamers bound to their protein target. Guided by chemical mapping, we systematically minimized an RNA aptamer (Lys1) selected against hen egg white lysozyme. The resultant 59-nucleotide compact aptamer (Lys1.2minE) retains nanomolar binding affinity and the ability to inhibit lysozyme's catalytic activity. Our 2.0-Å crystal structure of the aptamer-protein complex reveals a helical stem stabilizing two loops to form a protein binding platform that binds lysozyme distal to the catalytic cleft. This structure along with complementary solution analyses illuminate a novel protein-nucleic acid interface; (1) only 410 Å(2) of solvent accessible surface are buried by aptamer binding; (2) an unusually small fraction (∼18%) of the RNA-protein interaction is electrostatic, consistent with the limited protein phosphate backbone contacts observed in the structure; (3) a single Na(+) stabilizes the loops that constitute the protein-binding platform, and consistent with this observation, Lys1.2minE-lysozyme complex formation takes up rather than displaces cations at low ionic strength; (4) Lys1.2minE inhibits catalysis of large cell wall substrates but not catalysis of small model substrates; and (5) the helical stem of Lys1.2minE can be shortened to four base pairs (Lys1.2minF) without compromising binding affinity, yielding a 45-nucleotide aptamer whose structure may be an adaptable protein binding platform.

摘要

RNA 适体被开发为大分子和细胞功能的抑制剂、诊断工具和潜在的治疗药物。我们对这一新兴核酸-蛋白质复合物类别的物理性质的理解是有限的;只有少数结合其蛋白质靶标的适体的原子分辨率结构被报道。在化学作图的指导下,我们系统地最小化了一种针对鸡卵清溶菌酶的 RNA 适体(Lys1)。所得的 59 个核苷酸的紧凑适体(Lys1.2minE)保留了纳摩尔结合亲和力,并保持抑制溶菌酶催化活性的能力。我们 2.0Å 的适体-蛋白质复合物晶体结构揭示了一个螺旋茎稳定两个环,形成一个蛋白质结合平台,该平台结合溶菌酶远离催化裂缝。该结构以及互补的溶液分析阐明了一种新的蛋白质-核酸界面;(1)仅 410Å2 的溶剂可及表面被适体结合所埋藏;(2)RNA-蛋白质相互作用中只有一小部分(约 18%)是静电的,与结构中观察到的有限的蛋白质磷酸骨架接触一致;(3)一个单一的 Na+稳定构成蛋白质结合平台的环,与这一观察结果一致,Lys1.2minE-溶菌酶复合物的形成是占据而不是在低离子强度下取代阳离子;(4)Lys1.2minE 抑制大细胞壁底物的催化,但不抑制小模型底物的催化;(5)Lys1.2minE 的螺旋茎可以缩短到四个碱基(Lys1.2minF)而不影响结合亲和力,产生一个 45 个核苷酸的适体,其结构可能是一个可适应的蛋白质结合平台。

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