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SMN Tudor结构域的结构域边界定义及结晶

Definition of domain boundaries and crystallization of the SMN Tudor domain.

作者信息

Sprangers Remco, Selenko Philipp, Sattler Michael, Sinning Irmgard, Groves Matthew R

机构信息

Structural and Computational Biology, EMBL, Meyerhofstrasse 1, D-69012, Heidelberg, Germany.

出版信息

Acta Crystallogr D Biol Crystallogr. 2003 Feb;59(Pt 2):366-8. doi: 10.1107/s0907444902021406. Epub 2003 Jan 23.

Abstract

Spinal muscular atropy (SMA) is the major genetic disease leading to childhood mortality and is caused by mutations in or deletions of the smn1 gene. The human survival of motor neurons (SMN) protein encoded by this gene plays an important role in the assembly of snRNPs (small nuclear ribonucleoprotein complexes) via binding to the spliceosomal Sm proteins. The tails of these Sm proteins contain symmetrically dimethylated arginines that are recognized by the central SMN Tudor domain. To gain insight in the molecular basis of this specific interaction, the SMN Tudor domain has been crystallized. The rapid crystallization of the protein and the high stability of the crystals is facilitated by redefinition of domain boundaries based on NMR relaxation experiments and the previously determined solution structure. The crystals diffract to high resolution (1.8 A) and a complete data set has been collected from a hexagonal crystal form (P6(1)/P6(5)), with unit-cell parameters a = b = 27.65, c = 110.30 A, alpha = beta = 90, gamma = 120 degrees. Crystal soaks and co-crystallization with peptides derived from the Sm protein tails have been initiated. Molecular replacement with the NMR coordinates is under way.

摘要

脊髓性肌萎缩症(SMA)是导致儿童死亡的主要遗传性疾病,由运动神经元存活基因1(SMN1)的突变或缺失引起。该基因编码的人类运动神经元存活(SMN)蛋白通过与剪接体Sm蛋白结合,在小核核糖核蛋白复合物(snRNP)的组装中发挥重要作用。这些Sm蛋白的尾部含有对称二甲基化精氨酸,可被中央SMN Tudor结构域识别。为深入了解这种特异性相互作用的分子基础,已使SMN Tudor结构域结晶。基于核磁共振弛豫实验和先前确定的溶液结构对结构域边界进行重新定义,有助于蛋白质的快速结晶和晶体的高稳定性。晶体衍射分辨率高(1.8 Å),已从六方晶系晶体形式(P6(1)/P6(5))收集到完整数据集,晶胞参数a = b = 27.65,c = 110.30 Å,α = β = 90,γ = 120°。已开始用源自Sm蛋白尾部的肽进行晶体浸泡和共结晶实验。正在用核磁共振坐标进行分子置换。

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