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磷脂酶 D 通过调节 G 蛋白信号控制盘基网柄菌的发育。

Phospholipase D controls Dictyostelium development by regulating G protein signaling.

机构信息

Department of Biological Sciences, Hunter College, New York, New York 10065, USA.

出版信息

Cell Signal. 2011 Feb;23(2):335-43. doi: 10.1016/j.cellsig.2010.09.017. Epub 2010 Oct 13.

Abstract

Dictyostelium discoideum cells normally exist as individual amoebae, but will enter a period of multicellular development upon starvation. The initial stages of development involve the aggregation of individual cells, using cAMP as a chemoattractant. Chemotaxis is initiated when cAMP binds to its receptor, cAR1, and activates the associated G protein, Gα2βγ. However, chemotaxis will not occur unless there is a high density of starving cells present, as measured by high levels of the secreted quorum sensing molecule, CMF. We previously demonstrated that cells lacking PldB bypass the need for CMF and can aggregate at low cell density, whereas cells overexpressing pldB do not aggregate even at high cell density. Here, we found that PldB controlled both cAMP chemotaxis and cell sorting. PldB was also required by CMF to regulate G protein signaling. Specifically, CMF used PldB, to regulate the dissociation of Gα2 from Gβγ. Using fluorescence resonance energy transfer (FRET), we found that along with cAMP, CMF increased the dissociation of the G protein. In fact, CMF augmented the dissociation induced by cAMP. This augmentation was lost in cells lacking PldB. PldB appears to mediate the CMF signal through the production of phosphatidic acid, as exogenously added phosphatidic acid phenocopies overexpression of pldB. These results suggest that phospholipase D activity is required for CMF to alter the kinetics of cAMP-induced G protein signaling.

摘要

粘菌细胞通常以单个变形虫的形式存在,但在饥饿时会进入多细胞发育阶段。发育的初始阶段涉及到单个细胞的聚集,使用 cAMP 作为趋化引诱剂。当 cAMP 与其受体 cAR1 结合并激活相关的 G 蛋白 Gα2βγ 时,趋化作用就会开始。然而,除非存在高浓度的饥饿细胞(如通过高水平分泌的群体感应分子 CMF 测量),否则不会发生趋化作用。我们之前证明,缺乏 PldB 的细胞可以绕过对 CMF 的需求,并在低细胞密度下聚集,而过表达 pldB 的细胞即使在高细胞密度下也不会聚集。在这里,我们发现 PldB 控制 cAMP 趋化性和细胞分选。CMF 还需要 PldB 来调节 G 蛋白信号。具体来说,CMF 利用 PldB 调节 Gα2 与 Gβγ 的解离。使用荧光共振能量转移(FRET),我们发现与 cAMP 一起,CMF 增加了 G 蛋白的解离。事实上,CMF 增强了 cAMP 诱导的解离。在缺乏 PldB 的细胞中,这种增强作用消失了。PldB 似乎通过产生磷脂酸来介导 CMF 信号,因为外源性添加的磷脂酸模拟了 pldB 的过表达。这些结果表明,磷脂酶 D 活性是 CMF 改变 cAMP 诱导的 G 蛋白信号动力学所必需的。

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