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Local dynamics measured by hydrogen/deuterium exchange and mass spectrometry of creatine kinase digested by two proteases

机译:通过氢/氘交换和两种蛋白酶消化的肌酸激酶的质谱测定的局部动力学

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Hydrogen/deuterium exchange coupled to mass spectrometry has been used to investigate the structure and dynamics of native dimeric cytosolic muscle creatine kinase. The protein was incubated in D_2O for various time. After H/D exchange and rapid quenching of the reaction, the partially deuterated protein was cleaved in parallel by two different proteases (pepsin or type XIII protease from Aspergillus saitoi) to increase the sequence coverage and spatial resolution of deuterium incorporation. The resulting peptides were analyzed by liquid chromatog-raphy coupled to mass spectrometry. In comparison with the 3D structure of MM-CK, the analysis of the two independent proteolysis deu-teration patterns allowed us to get new insights into CK local dynamics as compared to a previous study using pepsin [Mazon et al. Protein Science 13 (2004) 476-486]. In particular, we obtained more information on the kinetics and extent of deuterium exchange in the N- and C-terminal extremities represented by the 1-22 and 362-380 pepsin peptides. Indeed, we observed a very different behaviour of the 1-12 and 13-22 type XIII protease peptides, and similarly for the 362-373 and 374-380 peptides. Moreover, comparison of the deuteration patterns of type XIII protease segments of the large 90-126 pepsin peptide led us to identify a small relatively dynamic region (108-114).
机译:氢/氘交换与质谱联用已用于研究天然二聚体胞质肌酸肌酸激酶的结构和动力学。蛋白质在D_2O中孵育各种时间。在H / D交换和反应快速淬灭后,部分氘化的蛋白质被两种不同的蛋白酶(胃蛋白酶或来自Saitogillus saitoi的XIII型蛋白酶)平行裂解,以增加序列覆盖率和氘掺入的空间分辨率。通过液相色谱-质谱联用分析所得的肽。与MM-CK的3D结构相比,与以前使用胃蛋白酶的研究相比,对两种独立的蛋白水解氘模式的分析使我们对CK局部动力学有了新的认识[Mazon等。蛋白质科学13(2004)476-486]。特别是,我们获得了有关以1-22和362-380胃蛋白酶肽为代表的N和C末端末端氘交换动力学和程度的更多信息。实际上,我们观察到1-12和13-22型XIII蛋白酶肽的行为截然不同,对于362-373和374-380肽也是如此。此外,比较大型90-126胃蛋白酶肽的XIII型蛋白酶区段的氘代模式,可以确定一个较小的相对动态区域(108-114)。

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