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Crystallographic studies on p21H-ras using the synchrotron Laue method: improvement of crystal quality and monitoring of the GTPase reaction at different time points

机译:使用同步加速器Laue方法对p21H-ras进行晶体学研究:在不同时间点改善晶体质量和监测GTp酶反应

摘要

The parameters affecting the crystal quality of complexes between p21H-ras and caged GTP have been investigated. The use of pure diastereomers of caged GTP complexed to the more stable p21(G12P)' mutant of p21 and the addition of n-octyl-[beta]-D-glucopyranoside improved the reproducibility and decreased the mosaicity of the crystals significantly. Furthermore, the crystallization technique was changed from the batch method to the sitting-drop technique. With the availability of a larger yield of well ordered crystals, it was possible to extend the time-resolved crystallographic investigations on p21H-ras. A structure of p21(G12P)':GTP could be obtained 2 min after photolytic removal of the cage group and led to the identification of a previously unidentified conformation for the so-called catalytically active loop L4. The refinement of five data sets collected within 2 min at different times (2-4, 11-13, 20-22, 30-32 and 90-92 min) after the initiation of the intrinsic GTPase reaction of the protein indicates that the synchrotron Laue method can be used to detect small structural changes and alternative conformations, but is presently limited in the analysis of larger rearrangements since these produce diffuse and broken electron density.
机译:研究了影响p21H-ras与笼状GTP之间复合物晶体质量的参数。使用笼状GTP的纯非对映异构体与p21的更稳定的p21(G12P)'突变体复合,并添加正辛基-β-D-吡喃葡萄糖苷,可显着提高可重复性并降低晶体的镶嵌性。此外,结晶技术从分批方法变为坐滴法。由于可以得到更高产量的有序晶体,因此有可能延长对p21H-ras的时间分辨晶体学研究。 p21(G12P)':GTP的结构可在光解去除笼基团后2分钟获得,并导致鉴定出所谓催化活性环L4先前未鉴定的构象。蛋白质内在GTPase反应启动后2分钟内在不同时间(2-4、11-13、20-22、30-32和90-92分钟)收集的五个数据集的细化表明,同步加速器劳厄方法可用于检测微小的结构变化和替代构象,但由于较大的重排会产生扩散和破坏的电子密度,因此目前在分析较大重排时受到限制。

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