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一种基因工程分子马达的结构。

Structure of a genetically engineered molecular motor.

作者信息

Kliche W, Fujita-Becker S, Kollmar M, Manstein D J, Kull F J

机构信息

Department of Biophysics, Max Planck Institute for Medical Research, Jahnstrasse 29, 69120 Heidelberg, Germany.

出版信息

EMBO J. 2001 Jan 15;20(1-2):40-6. doi: 10.1093/emboj/20.1.40.

Abstract

Molecular motors move unidirectionally along polymer tracks, producing movement and force in an ATP-dependent fashion. They achieve this by amplifying small conformational changes in the nucleotide-binding region into force-generating movements of larger protein domains. We present the 2.8 A resolution crystal structure of an artificial actin-based motor. By combining the catalytic domain of myosin II with a 130 A conformational amplifier consisting of repeats 1 and 2 of alpha-actinin, we demonstrate that it is possible to genetically engineer single-polypeptide molecular motors with precisely defined lever arm lengths and specific motile properties. Furthermore, our structure shows the consequences of mutating a conserved salt bridge in the nucleotide-binding region. Disruption of this salt bridge, which is known to severely inhibit ATP hydrolysis activity, appears to interfere with formation of myosin's catalytically active 'closed' conformation. Finally, we describe the structure of alpha-actinin repeats 1 and 2 as being composed of two rigid, triple-helical bundles linked by an uninterrupted alpha-helix. This fold is very similar to the previously described structures of alpha-actinin repeats 2 and 3, and alpha-spectrin repeats 16 and 17.

摘要

分子马达沿着聚合物轨道单向移动,以ATP依赖的方式产生运动和力。它们通过将核苷酸结合区域的小构象变化放大为更大蛋白质结构域的力产生运动来实现这一点。我们展示了一种基于肌动蛋白的人工马达的2.8埃分辨率晶体结构。通过将肌球蛋白II的催化结构域与由α-辅肌动蛋白的重复序列1和2组成的130埃构象放大器相结合,我们证明可以通过基因工程构建具有精确定义的杠杆臂长度和特定运动特性的单多肽分子马达。此外,我们的结构展示了核苷酸结合区域中一个保守盐桥突变的后果。已知破坏这个盐桥会严重抑制ATP水解活性,它似乎会干扰肌球蛋白催化活性“闭合”构象的形成。最后,我们描述了α-辅肌动蛋白重复序列1和2的结构,其由两个刚性的三螺旋束通过一个不间断的α-螺旋连接而成。这种折叠与先前描述的α-辅肌动蛋白重复序列2和3以及α-血影蛋白重复序列16和17的结构非常相似。

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