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肌动蛋白调节激酶在胞吞作用和酵母 epsin 磷酸化中的体内作用。

In vivo role for actin-regulating kinases in endocytosis and yeast epsin phosphorylation.

作者信息

Watson H A, Cope M J, Groen A C, Drubin D G, Wendland B

机构信息

Department of Biology, The Johns Hopkins University, Baltimore, Maryland 21218, USA.

出版信息

Mol Biol Cell. 2001 Nov;12(11):3668-79. doi: 10.1091/mbc.12.11.3668.

Abstract

The yeast actin-regulating kinases Ark1p and Prk1p are signaling proteins localized to cortical actin patches, which may be sites of endocytosis. Interactions between the endocytic proteins Pan1p and End3p may be regulated by Prk1p-dependent threonine phosphorylation of Pan1p within the consensus sequence [L/I]xxQxTG. We identified two Prk1p phosphorylation sites within the Pan1p-binding protein Ent1p, a yeast epsin homologue, and demonstrate Prk1p-dependent phosphorylation of both threonines. Converting both threonines to either glutamate or alanine mimics constitutively phosphorylated or dephosphorylated Ent1p, respectively. Synthetic growth defects were observed in a pan1-20 ENT1(EE) double mutant, suggesting that Ent1p phosphorylation negatively regulates the formation/activity of a Pan1p-Ent1p complex. Interestingly, pan1-20 ent2 Delta but not pan1-20 ent1 Delta double mutants had improved growth and endocytosis over the pan1-20 mutant. We found that actin-regulating Ser/Thr kinase (ARK) mutants exhibit endocytic defects and that overexpressing either wild-type or alanine-substituted Ent1p partially suppressed phenotypes associated with loss of ARK kinases, including growth, endocytosis, and actin localization defects. Consistent with synthetic growth defects of pan1-20 ENT1(EE) cells, overexpressing glutamate-substituted Ent1p was deleterious to ARK mutants. Surprisingly, overexpressing the related Ent2p protein could not suppress ARK kinase mutant phenotypes. These results suggest that Ent1p and Ent2p are not completely redundant and may perform opposing functions in endocytosis. These data support the model that, as for clathrin-dependent recycling of synaptic vesicles, yeast endocytic protein phosphorylation inhibits endocytic functions.

摘要

酵母肌动蛋白调节激酶Ark1p和Prk1p是定位于皮质肌动蛋白斑块的信号蛋白,皮质肌动蛋白斑块可能是内吞作用的位点。内吞蛋白Pan1p和End3p之间的相互作用可能受Prk1p依赖的Pan1p在共有序列[L/I]xxQxTG内的苏氨酸磷酸化调控。我们在Pan1p结合蛋白Ent1p(一种酵母epsin同源物)中鉴定出两个Prk1p磷酸化位点,并证明这两个苏氨酸均发生Prk1p依赖的磷酸化。将这两个苏氨酸分别转换为谷氨酸或丙氨酸分别模拟了组成型磷酸化或去磷酸化的Ent1p。在pan1-20 ENT1(EE)双突变体中观察到合成生长缺陷,表明Ent1p磷酸化负向调节Pan1p-Ent1p复合物的形成/活性。有趣的是,pan1-20 ent2Δ双突变体而非pan1-20 ent1Δ双突变体相较于pan1-20突变体具有改善的生长和内吞作用。我们发现肌动蛋白调节丝氨酸/苏氨酸激酶(ARK)突变体表现出内吞缺陷,并且过表达野生型或丙氨酸取代的Ent1p可部分抑制与ARK激酶缺失相关的表型,包括生长、内吞作用和肌动蛋白定位缺陷。与pan1-20 ENT1(EE)细胞的合成生长缺陷一致,过表达谷氨酸取代的Ent1p对ARK突变体有害。令人惊讶的是,过表达相关的Ent2p蛋白不能抑制ARK激酶突变体表型。这些结果表明Ent1p和Ent2p并非完全冗余,可能在内吞作用中发挥相反的功能。这些数据支持这样的模型,即对于网格蛋白依赖的突触小泡循环,酵母内吞蛋白磷酸化抑制内吞功能。

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