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本文引用的文献

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Cell Polarity in Yeast.酵母细胞极性。
Annu Rev Cell Dev Biol. 2017 Oct 6;33:77-101. doi: 10.1146/annurev-cellbio-100616-060856. Epub 2017 Aug 7.
2
Offline pentafluorophenyl (PFP)-RP prefractionation as an alternative to high-pH RP for comprehensive LC-MS/MS proteomics and phosphoproteomics.离线五氟苯基(PFP)-反相预分级分离作为高pH值反相用于全面液相色谱-串联质谱蛋白质组学和磷酸化蛋白质组学分析的替代方法
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Phosphatases Generate Signal Specificity Downstream of Ssp1 Kinase in Fission Yeast.磷酸酶在裂殖酵母中Ssp1激酶下游产生信号特异性。
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Identification of Candidate Cyclin-dependent kinase 1 (Cdk1) Substrates in Mitosis by Quantitative Phosphoproteomics.通过定量磷酸化蛋白质组学鉴定有丝分裂中潜在的细胞周期蛋白依赖性激酶1(Cdk1)底物
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Quantitative phosphoproteomics reveals new roles for the protein phosphatase PP6 in mitotic cells.定量磷酸化蛋白质组学揭示了蛋白磷酸酶PP6在有丝分裂细胞中的新作用。
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Quantitative phosphoproteomics reveals pathways for coordination of cell growth and division by the conserved fission yeast kinase pom1.定量磷酸化蛋白质组学揭示了保守的裂殖酵母激酶pom1协调细胞生长和分裂的途径。
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8
The Cdc15 and Imp2 SH3 domains cooperatively scaffold a network of proteins that redundantly ensure efficient cell division in fission yeast.Cdc15和Imp2的SH3结构域协同搭建一个蛋白质网络,该网络以冗余方式确保裂殖酵母中的细胞分裂高效进行。
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ProteomeXchange provides globally coordinated proteomics data submission and dissemination.蛋白质组学交换库提供全球协调的蛋白质组学数据提交和传播服务。
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10
Dueling kinases regulate cell size at division through the SAD kinase Cdr2.相互竞争的激酶通过SAD激酶Cdr2在细胞分裂时调节细胞大小。
Curr Biol. 2014 Feb 17;24(4):428-33. doi: 10.1016/j.cub.2014.01.009. Epub 2014 Feb 6.

连接裂殖酵母细胞极性和分裂的保守蛋白激酶 Ssp1、Kin1 和 Pom1 的机制。

Mechanisms Connecting the Conserved Protein Kinases Ssp1, Kin1, and Pom1 in Fission Yeast Cell Polarity and Division.

机构信息

Department of Biochemistry and Cell Biology, The Geisel School of Medicine at Dartmouth, Hanover, NH 03755, USA.

Department of Biochemistry and Cell Biology, The Geisel School of Medicine at Dartmouth, Hanover, NH 03755, USA; Norris Cotton Cancer Center, The Geisel School of Medicine at Dartmouth, Lebanon, NH 03756, USA.

出版信息

Curr Biol. 2018 Jan 8;28(1):84-92.e4. doi: 10.1016/j.cub.2017.11.034. Epub 2017 Dec 14.

DOI:10.1016/j.cub.2017.11.034
PMID:29249658
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC5760279/
Abstract

Connections between the protein kinases that function within complex cell polarity networks are poorly understood. Rod-shaped fission yeast cells grow in a highly polarized manner, and genetic screens have identified many protein kinases, including the CaMKK-like Ssp1 and the MARK/PAR-1 family kinase Kin1, that are required for polarized growth and cell shape, but their functional mechanisms and connections have been unknown [1-5]. We found that Ssp1 promotes cell polarity by phosphorylating the activation loop of Kin1. Kin1 regulates cell polarity and cytokinesis through unknown mechanisms [4-7]. We performed a large-scale phosphoproteomic screen and found that Kin1 phosphorylates itself and Pal1 to promote growth at cell tips, and these proteins are interdependent for localization to growing cell tips. Additional Kin1 substrates for cell polarity and cytokinesis (Tea4, Mod5, Cdc15, and Cyk3) were also phosphorylated by a second kinase, the DYRK family member Pom1 [8]. Kin1 and Pom1 were enriched at opposite ends of growing cells, and they phosphorylated largely non-overlapping sites on shared substrates. Combined inhibition of both Kin1and Pom1 led to synthetic defects in their shared substrates Cdc15 and Cyk3, confirming a non-redundant functional connection through shared substrates. These findings uncover a new Ssp1-Kin1 signaling pathway, and define its functional and mechanistic connection with Pom1 signaling for cell polarity and cytokinesis. These kinases are conserved in many eukaryotes including humans, suggesting that similar connections and mechanisms might operate in a broad range of cells.

摘要

细胞极性复杂网络中发挥作用的蛋白激酶之间的联系还知之甚少。杆状裂殖酵母细胞以高度极化的方式生长,遗传筛选已经鉴定出许多蛋白激酶,包括钙调蛋白激酶样 Ssp1 和 MARK/PAR-1 家族激酶 Kin1,它们对于极化生长和细胞形状是必需的,但它们的功能机制和联系还不清楚[1-5]。我们发现 Ssp1 通过磷酸化 Kin1 的激活环促进细胞极性。Kin1 通过未知机制调节细胞极性和胞质分裂[4-7]。我们进行了大规模的磷酸化蛋白质组学筛选,发现 Kin1 自身和 Pal1 磷酸化以促进细胞尖端的生长,这些蛋白质对于定位到生长中的细胞尖端是相互依赖的。细胞极性和胞质分裂的其他 Kin1 底物(Tea4、Mod5、Cdc15 和 Cyk3)也被 DYRK 家族成员 Pom1 磷酸化[8]。Kin1 和 Pom1 在生长细胞的相对端富集,它们在共享底物上磷酸化的位点大部分不重叠。同时抑制 Kin1 和 Pom1 导致它们共同底物 Cdc15 和 Cyk3 的合成缺陷,证实通过共享底物存在非冗余的功能联系。这些发现揭示了一个新的 Ssp1-Kin1 信号通路,并定义了其与 Pom1 信号通路在细胞极性和胞质分裂中的功能和机制联系。这些激酶在许多真核生物中包括人类中都保守,表明类似的联系和机制可能在广泛的细胞中运作。