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天然兔肌酸激酶动力学的氢/氘交换研究。

Hydrogen/deuterium exchange studies of native rabbit MM-CK dynamics.

作者信息

Mazon Hortense, Marcillat Olivier, Forest Eric, Vial Christian

机构信息

UMR 5013 CNRS, Université Claude Bernard Lyon I, 43 boulevard du 11 Novembre 1918, 69622 Villeurbanne cedex, France.

出版信息

Protein Sci. 2004 Feb;13(2):476-86. doi: 10.1110/ps.03380604.

Abstract

Creatine kinase (CK) isoenzymes catalyse the reversible transfer of a phosphoryl group from ATP onto creatine. This reaction plays a very important role in the regulation of intracellular ATP concentrations in excitable tissues. CK isoenzymes are highly resistant to proteases in native conditions. To appreciate localized backbone dynamics, kinetics of amide hydrogen exchange with deuterium was measured by pulse-labeling the dimeric cytosolic muscle CK isoenzyme. Upon exchange, the protein was digested with pepsin, and the deuterium content of the resulting peptides was determined by liquid chromatography coupled to mass spectrometry (MS). The deuteration kinetics of 47 peptides identified by MS/MS and covering 96% of the CK backbone were analyzed. Four deuteration patterns have been recognized: The less deuterated peptides are located in the saddle-shaped core of CK, whereas most of the highly deuterated peptides are close to the surface and located around the entrance to the active site. Their exchange kinetics are discussed by comparison with the known secondary and tertiary structures of CK with the goal to reveal the conformational dynamics of the protein. Some of the observed dynamic motions may be linked to the conformational changes associated with substrate binding and catalytic mechanism.

摘要

肌酸激酶(CK)同工酶催化磷酸基团从ATP可逆地转移到肌酸上。该反应在可兴奋组织中细胞内ATP浓度的调节中起着非常重要的作用。在天然条件下,CK同工酶对蛋白酶具有高度抗性。为了了解局部主链动力学,通过脉冲标记二聚体胞质肌肉CK同工酶来测量酰胺氢与氘的交换动力学。交换后,用胃蛋白酶消化蛋白质,并通过液相色谱-质谱联用(MS)测定所得肽段的氘含量。分析了通过MS/MS鉴定的47个肽段的氘化动力学,这些肽段覆盖了CK主链的96%。已识别出四种氘化模式:氘化程度较低的肽段位于CK的鞍形核心中,而大多数高度氘化的肽段靠近表面且位于活性位点入口周围。通过与已知的CK二级和三级结构进行比较来讨论它们的交换动力学,目的是揭示蛋白质的构象动力学。一些观察到的动态运动可能与底物结合和催化机制相关的构象变化有关。

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