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肌球蛋白表面环4调节原肌球蛋白对肌动球蛋白1b ATP酶活性的抑制作用。

Myosin surface loop 4 modulates inhibition of actomyosin 1b ATPase activity by tropomyosin.

作者信息

Lieto-Trivedi Alena, Dash Sheffali, Coluccio Lynne M

机构信息

Boston Biomedical Research Institute, 64 Grove Street, Watertown, Massachusetts 02472, USA.

出版信息

Biochemistry. 2007 Mar 13;46(10):2779-86. doi: 10.1021/bi602439f. Epub 2007 Feb 14.

DOI:10.1021/bi602439f
PMID:17298083
Abstract

Structural studies of the class I myosin, MyoE, led to the predictions that loop 4, a surface loop near the actin-binding region that is longer in class I myosins than in other myosin subclasses, might limit binding of myosins I to actin when actin-binding proteins, like tropomyosin, are present, and might account for the exclusion of myosin I from stress fibers. To test these hypotheses, mutant molecules of the related mammalian class I myosin, Myo1b, in which loop 4 was truncated (from an amino acid sequence of RMNGLDES to NGLD) or replaced with the shorter and distinct loop 4 found in Dictyostelium myosin II (GAGEGA), were expressed in vitro and their interaction with actin and with actin-tropomyosin was tested. Saturating amounts of expressed fibroblast tropomyosin-2 resulted in a decrease in the maximum actin-activated Mg2+-ATPase activity of wild-type Myo1b but had little or no effect on the actin-activated Mg2+-ATPase activity of the two mutants. In motility assays, few actin filaments bound tightly to Myo1b-WT-coated cover slips when tropomyosin-2 was present, whereas actin filaments both bound and were translocated by Myo1b-NGLD or Myo1b-GAGEGA in both the presence and absence of tropomyosin-2. When expressed in mammalian cells, like the wild type, the mutant myosins were largely excluded from tropomyosin-containing actin filaments, indicating that in the cell additional factors besides loop 4 determine targeting of myosins I to specific subpopulations of actin filaments.

摘要

对I类肌球蛋白MyoE的结构研究得出如下预测:环4是肌动蛋白结合区域附近的一个表面环,在I类肌球蛋白中比在其他肌球蛋白亚类中更长,当存在肌动蛋白结合蛋白(如原肌球蛋白)时,它可能会限制I类肌球蛋白与肌动蛋白的结合,并且可能是I类肌球蛋白被排除在应力纤维之外的原因。为了验证这些假设,在体外表达了相关的哺乳动物I类肌球蛋白Myo1b的突变分子,其中环4被截短(从RMNGLDES的氨基酸序列变为NGLD)或被盘基网柄菌肌球蛋白II中较短且不同的环4(GAGEGA)取代,并测试了它们与肌动蛋白以及肌动蛋白 - 原肌球蛋白的相互作用。饱和量的成纤维细胞原肌球蛋白 - 2导致野生型Myo1b的最大肌动蛋白激活的Mg2 + -ATP酶活性降低,但对两个突变体的肌动蛋白激活的Mg2 + -ATP酶活性几乎没有影响。在运动分析中,当存在原肌球蛋白 - 2时,很少有肌动蛋白丝紧密结合到Myo1b - WT包被的盖玻片上,而在存在和不存在原肌球蛋白 - 2的情况下,肌动蛋白丝都能与Myo1b - NGLD或Myo1b - GAGEGA结合并发生移位。当在哺乳动物细胞中表达时,与野生型一样,突变型肌球蛋白在很大程度上被排除在含有原肌球蛋白的肌动蛋白丝之外,这表明在细胞中除了环4之外还有其他因素决定I类肌球蛋白靶向特定的肌动蛋白丝亚群。

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