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在反应性巯基区域具有甘氨酸到丙氨酸突变的盘基网柄菌肌球蛋白运动结构域的动力学分析。

Kinetic analysis of Dictyostelium discoideum myosin motor domains with glycine-to-alanine mutations in the reactive thiol region.

作者信息

Batra R, Geeves M A, Manstein D J

机构信息

Max-Planck-Institut für Medizinische Forschung, Jahnstr. 29, D-69120 Heidelberg, Germany.

出版信息

Biochemistry. 1999 May 11;38(19):6126-34. doi: 10.1021/bi982251e.

DOI:10.1021/bi982251e
PMID:10320339
Abstract

Three conserved glycine residues in the reactive thiol region of Dictyostelium discoideummyosin II were replaced by alanine residues. The resulting mutants G680A, G684A, and G691A were expressed in the soluble myosin head fragment M761-2R [Anson, M., Geeves, M. A., Kurzawa, S. E., and Manstein, D. J. (1996) EMBO J. 15, 6069-6074] and characterized using transient kinetic methods. Mutant G691A showed no major alterations except for a marked increase in basal Mg2+-ATPase activity. Phosphate release seemed to be facilitated by this mutation, and the addition of actin to G691A stimulated ATP turnover not more than 3-fold. In comparison to M761-2R, mutant constructs G691A and G684A showed a 4-fold reduction in the rate of the ATP cleavage step. Most other changes in the kinetic properties of G684A were small ( approximately 2-fold). In contrast, substitution of G680 by an alanine residue led to large changes in nucleotide binding. Compared to M761-2R, rates of nucleotide binding were 20-30-fold slower and the affinity for mantADP was approximately 10-fold increased due to a 200-fold reduction in the dissociation rate constant of mantADP. The ATP-induced dissociation of actin from the acto.680A complex was normal, but the communication between ADP and actin binding was altered such that the two sites are thermodynamically uncoupled but kinetically actin still accelerates ADP release.

摘要

将盘基网柄菌肌球蛋白II反应性巯基区域中的三个保守甘氨酸残基替换为丙氨酸残基。所得突变体G680A、G684A和G691A在可溶性肌球蛋白头部片段M761 - 2R中表达[安森,M.,吉夫斯,M. A.,库尔扎瓦,S. E.,和曼斯坦,D. J.(1996年)《欧洲分子生物学组织杂志》15,6069 - 6074],并使用瞬态动力学方法进行表征。除了基础Mg2 + - ATP酶活性显著增加外,突变体G691A没有显示出重大改变。该突变似乎促进了磷酸释放,并且向G691A中添加肌动蛋白对ATP周转的刺激不超过3倍。与M761 - 2R相比,突变体构建体G691A和G684A在ATP裂解步骤的速率上降低了4倍。G684A动力学性质的大多数其他变化较小(约2倍)。相比之下,用丙氨酸残基取代G680导致核苷酸结合发生巨大变化。与M761 - 2R相比,核苷酸结合速率慢20 - 30倍,并且由于mantADP解离速率常数降低200倍,对mantADP的亲和力增加了约10倍。ATP诱导肌动蛋白从肌动蛋白.680A复合物中解离是正常的,但ADP与肌动蛋白结合之间的通讯发生了改变,使得这两个位点在热力学上解偶联,但在动力学上肌动蛋白仍加速ADP释放。

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