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核糖核酸酶A荧光衍生物的晶体结构

Crystal structure of a fluorescent derivative of RNase A.

作者信息

Baudet-Nessler S, Jullien M, Crosio M P, Janin J

机构信息

Laboratoire de Biologie Structurale, UMR 9920 CNRS-Université Paris-Sud, Orsay, France.

出版信息

Biochemistry. 1993 Aug 24;32(33):8457-64.

PMID:8357795
Abstract

The crystal structure of RNase A chemically modified with the fluorescent probe, N-[[(iodoacetyl)-amino]ethyl]-5-naphthylamine-1-sulfonic acid (1,5-IAENS), has been solved and refined to high resolution. It yields information on the mode of binding, the mobility of a probe commonly used in spectroscopic studies, and anion binding sites in RNase A. Trigonal crystals of the fluorescent derivative grown in sodium or cesium chloride and ammonium sulfate, pH 5.1, were nearly isomorphous with those of a semisynthetic RNase [DeMel, et al. (1992) J. Biol. Chem. 267, 247-256]. Refinement starting from semisynthetic RNase led to a model with R = 20% against 1.7-A diffraction data from crystals in ammonium sulfate and another model with R = 17% against 1.9-A data taken in the presence of 3 M NaCl. The second model contains three chloride ions: one is at the active site, and the other two are at molecular interfaces. Otherwise, the two models are very similar. The fluorophore has very little effect on the protein conformation. It is found to be covalently attached to the active site His-12 with the naphthyl group stacked on the imidazole ring of His-119. It remains largely accessible to solvent and in a polar environment on the protein surface, even though the fluorescence emission spectrum is blue shifted as it is in nonpolar solvents.

摘要

用荧光探针N-[[(碘乙酰基)-氨基]乙基]-5-萘胺-1-磺酸(1,5-IAENS)化学修饰的核糖核酸酶A(RNase A)的晶体结构已被解析并精修至高分辨率。它提供了关于结合模式、光谱研究中常用探针的流动性以及RNase A中阴离子结合位点的信息。在pH 5.1的氯化钠、氯化铯和硫酸铵中生长的荧光衍生物的三角晶体与一种半合成RNase的晶体几乎同晶型[DeMel等人(1992年)《生物化学杂志》267, 247 - 256]。从半合成RNase开始精修得到一个模型,对于来自硫酸铵晶体的1.7 Å衍射数据,R值为20%;另一个模型对于在3 M氯化钠存在下获取的1.9 Å数据,R值为17%。第二个模型包含三个氯离子:一个在活性位点,另外两个在分子界面。否则,这两个模型非常相似。荧光团对蛋白质构象影响很小。发现它通过萘基堆叠在His - 119的咪唑环上与活性位点的His - 12共价连接。尽管其荧光发射光谱如在非极性溶剂中一样发生蓝移,但它在很大程度上仍可接触溶剂且处于蛋白质表面的极性环境中。

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