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DNase-I 结合环的特异性切割显著降低了肌动蛋白的热稳定性。

Specific cleavage of the DNase-I binding loop dramatically decreases the thermal stability of actin.

机构信息

A. N. Bach Institute of Biochemistry, Russian Academy of Sciences, Moscow, Russia.

出版信息

FEBS J. 2010 Sep;277(18):3812-22. doi: 10.1111/j.1742-4658.2010.07782.x. Epub 2010 Aug 13.

DOI:10.1111/j.1742-4658.2010.07782.x
PMID:20718862
Abstract

Differential scanning calorimetry was used to investigate the thermal unfolding of actin specifically cleaved within the DNaseI-binding loop between residues Met47-Gly48 or Gly42-Val43 by two bacterial proteases, subtilisin or ECP32/grimelysin (ECP), respectively. The results obtained show that both cleavages strongly decreased the thermal stability of monomeric actin with either ATP or ADP as a bound nucleotide. An even more pronounced difference in the thermal stability between the cleaved and intact actin was observed when both actins were polymerized into filaments. Similar to intact F-actin, both cleaved F-actins were significantly stabilized by phalloidin and aluminum fluoride; however, in all cases, the thermal stability of the cleaved F-actins was much lower than that of intact F-actin, and the stability of ECP-cleaved F-actin was lower than that of subtilisin-cleaved F-actin. These results confirm that the DNaseI-binding loop is involved in the stabilization of the actin structure, both in monomers and in the filament subunits, and suggest that the thermal stability of actin depends, at least partially, on the conformation of the nucleotide-binding cleft. Moreover, an additional destabilization of the unstable cleaved actin upon ATP/ADP replacement provides experimental evidence for the highly dynamic actin structure that cannot be simply open or closed, but rather should be considered as being able to adopt multiple conformations.

摘要

差示扫描量热法被用于研究两种细菌蛋白酶,枯草杆菌蛋白酶或 ECP32/grimelysin(ECP)分别在 Met47-Gly48 或 Gly42-Val43 残基之间的 DNaseI 结合环内特异性切割的肌动蛋白的热变性。结果表明,两种切割都强烈降低了单体肌动蛋白与 ATP 或 ADP 结合时的热稳定性。当两种肌动蛋白聚合成长丝时,观察到切割和完整肌动蛋白之间的热稳定性差异更加明显。与完整的 F-肌动蛋白相似,两种切割的 F-肌动蛋白都被鬼笔环肽和氟铝酸钠显著稳定;然而,在所有情况下,切割的 F-肌动蛋白的热稳定性都远低于完整的 F-肌动蛋白,而 ECP 切割的 F-肌动蛋白的稳定性低于枯草杆菌蛋白酶切割的 F-肌动蛋白。这些结果证实,DNaseI 结合环参与了肌动蛋白结构的稳定,无论是单体还是在纤维亚基中,并且表明肌动蛋白的热稳定性至少部分取决于核苷酸结合裂缝的构象。此外,ATP/ADP 取代后不稳定切割肌动蛋白的进一步失稳提供了实验证据,证明了肌动蛋白的高度动态结构不能简单地打开或关闭,而应该被认为能够采用多种构象。

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