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酿酒酵母中Arp2/3复合物肌动蛋白成核机制及其成核促进因子的不同作用剖析

Dissection of Arp2/3 complex actin nucleation mechanism and distinct roles for its nucleation-promoting factors in Saccharomyces cerevisiae.

作者信息

D'Agostino Jessica L, Goode Bruce L

机构信息

Department of Biology, Brandeis University, Waltham, Massachusetts 02454, USA.

出版信息

Genetics. 2005 Sep;171(1):35-47. doi: 10.1534/genetics.105.040634.

Abstract

Actin nucleation by the Arp2/3 complex is under tight control, remaining inactive until stimulation by nucleation-promoting factors (NPFs). Although multiple NPFs are expressed in most cell types, little is known about how they are coordinated and whether they perform similar or distinct functions. We examined genetic relationships among the four S. cerevisiae NPFs. Combining las17delta with pan1-101 or myo3delta myo5delta was lethal at all temperatures, whereas combining pan1-101 with myo3delta myo5delta showed no genetic interaction and abp1delta partially suppressed las17delta. These data suggest that NPFs have distinct and overlapping functions in vivo. We also tested genetic interactions between each NPF mutant and seven different temperature-sensitive arp2 alleles and purified mutant Arp2/3 complexes to compare their activities. Two arp2 alleles with mutations at the barbed end were severely impaired in nucleation, providing the first experimental evidence that Arp2 nucleates actin at its barbed end in vitro and in vivo. Another arp2 allele caused partially unregulated ("leaky") nucleation in the absence of NPFs. Combining this mutant with a partially unregulated allele in a different subunit of Arp2/3 complex was lethal, suggesting that cells cannot tolerate high levels of unregulated activity. Genetic interactions between arp2 alleles and NPF mutants point to Abp1 having an antagonistic role with respect to other NPFs, possibly serving to attenuate their stronger activities. In support of this model, Abp1 binds strongly to Arp2/3 complex, yet has notably weak nucleation-promoting activity and inhibits Las17 activity on Arp2/3 complex in a dose-responsive manner.

摘要

Arp2/3复合体介导的肌动蛋白成核受到严格调控,在成核促进因子(NPFs)刺激之前一直处于无活性状态。尽管大多数细胞类型中都表达多种NPFs,但对于它们如何协同作用以及它们执行的功能是相似还是不同,我们知之甚少。我们研究了酿酒酵母中四种NPFs之间的遗传关系。在所有温度下,将las17缺失与pan1 - 101或myo3缺失myo5缺失相结合都是致死的,而将pan1 - 101与myo3缺失myo5缺失相结合则未显示出遗传相互作用,并且abp1缺失部分抑制了las17缺失。这些数据表明NPFs在体内具有不同但又重叠的功能。我们还测试了每个NPF突变体与七个不同的温度敏感型arp2等位基因之间的遗传相互作用,并纯化了突变的Arp2/3复合体以比较它们的活性。两个在尖端有突变的arp2等位基因在成核方面严重受损,这首次提供了实验证据,表明Arp2在体外和体内均在其尖端介导肌动蛋白成核。另一个arp2等位基因在没有NPFs的情况下导致部分不受调控(“渗漏”)的成核。将这个突变体与Arp2/3复合体不同亚基中的一个部分不受调控的等位基因相结合是致死的,这表明细胞无法耐受高水平的不受调控的活性。arp2等位基因与NPF突变体之间的遗传相互作用表明,Abp1相对于其他NPFs具有拮抗作用,可能是为了减弱它们更强的活性。支持这一模型的是,Abp1与Arp2/3复合体紧密结合,但成核促进活性明显较弱,并以剂量反应方式抑制Las17对Arp2/3复合体的活性。

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