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酵母天冬氨酸-tRNA天冬氨酸合成酶:晶体复合物

Yeast tRNAAsp-aspartyl-tRNA synthetase: the crystalline complex.

作者信息

Moras D, Lorber B, Romby P, Ebel J P, Giegé R, Lewit-Bentley A, Roth M

机构信息

Institut de Biologie Moléculaire et Cellulaire du CNRS, Strasbourg, France.

出版信息

J Biomol Struct Dyn. 1983 Oct;1(1):209-23. doi: 10.1080/07391102.1983.10507435.

Abstract

Aspartyl-tRNA synthetase from yeast, a dimer of molecular weight 125,000 and its cognate tRNA (Mr = 24,160) were co-crystallized using ammonium sulfate as precipitant agent. The presence in the crystals of both components in the two-to-one stoichiometric ratio was demonstrated by electrophoresis, biological activity assays and crystallographic data. Crystals belong to the cubic space group I432 with cell parameter of 354 A and one complex particle per asymmetric unit. The solvent content of about 78% is favorable for a low resolution structural investigation. By exchanging H2O for D2O in mother liquors, advantage can be taken from contrast variation techniques with neutron radiations. Diffraction data to 20 A resolution were measured at five different contrasts, two of them being close to the theoretical matching point of RNA and protein in the presence of ammonium sulfate. The experimental extinction of the diffracted signal was observed to be close to 36% D2O, significantly different from the predicted value of 41%. The phenomenon can be explained by the existence of a large interface region between the two tRNAs and the enzyme. These parts of the molecules are hidden from the solvent and their protons are less easily exchangeable. Accessibility studies toward chemicals of tRNAAsp in solution and in the presence of synthetase are in agreement with such a model.

摘要

来自酵母的天冬氨酰 - tRNA合成酶(分子量为125,000的二聚体)及其同源tRNA(Mr = 24,160)以硫酸铵作为沉淀剂进行了共结晶。通过电泳、生物活性测定和晶体学数据证明了晶体中两种组分以二比一的化学计量比存在。晶体属于立方空间群I432,晶胞参数为354 Å,每个不对称单元有一个复合颗粒。约78%的溶剂含量有利于进行低分辨率结构研究。通过在母液中将H2O换成D2O,可以利用中子辐射的对比变化技术。在五个不同的对比度下测量了分辨率达20 Å的衍射数据,其中两个接近在硫酸铵存在下RNA和蛋白质的理论匹配点。观察到衍射信号的实验消光接近36% D2O,与预测值41%有显著差异。这种现象可以通过两个tRNA与酶之间存在大的界面区域来解释。分子的这些部分被溶剂屏蔽,其质子不易交换。对溶液中和存在合成酶时tRNAAsp对化学物质的可及性研究与这样的模型一致。

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