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活细胞中Gα(q)与磷脂酶Cβ1之间的稳定关联。

Stable association between G alpha(q) and phospholipase C beta 1 in living cells.

作者信息

Dowal Louisa, Provitera Paxton, Scarlata Suzanne

机构信息

Department of Physiology and Biophysics, State University of New York, Stony Brook, New York 11794-8661, USA.

出版信息

J Biol Chem. 2006 Aug 18;281(33):23999-4014. doi: 10.1074/jbc.M512330200. Epub 2006 Jun 5.

DOI:10.1074/jbc.M512330200
PMID:16754659
Abstract

Signal transduction through G alpha(q) involves stimulation of phospholipase C beta (PLC beta) that results in increased intracellular Ca2+ and activation of protein kinase C. We have measured complex formation between G alpha(q) and PLC beta1 in vitro and in living PC12 and HEK293 cells by fluorescence resonance energy transfer. In vitro measurements show that PLC beta1 will bind to G alpha(q)(guanosine 5'-3-O-(thio)triphosphate) and also to G alpha(q)(GDP), and the latter association has a different protein-protein orientation. In cells, image analysis of fluorescent-tagged proteins shows that G alpha(q) is localized almost entirely to the plasma membrane, whereas PLC beta1 has a significant cytosolic population. By using fluorescence resonance energy transfer, we found that these proteins are pre-associated in the unstimulated state in PC12 and HEK293 cells. By determining the cellular levels of the two proteins in transfected versus nontransfected cells, we found that under our conditions overexpression should not significantly promote complex formation. G alpha(q)-PLC beta1 complexes are observed in both single cell measurements and measurements of a large (i.e. 10(6)) cell suspension. The high level (approximately 40% maximum) of FRET is surprising considering that G alpha(q) is more highly expressed than PLC beta1 and that not all PLC beta1 is plasma membrane-localized. Our measurements suggest a model in which G proteins and effectors can exist in stable complexes prior to activation and that activation is achieved through changes in intermolecular interactions rather than diffusion and association. These pre-formed complexes in turn give rise to rapid, localized signals.

摘要

通过Gα(q)的信号转导涉及磷脂酶Cβ(PLCβ)的激活,这会导致细胞内Ca2+增加和蛋白激酶C的活化。我们通过荧光共振能量转移在体外以及活的PC12和HEK293细胞中测量了Gα(q)与PLCβ1之间的复合物形成。体外测量表明,PLCβ1能与Gα(q)(鸟苷5'-3-O-(硫代)三磷酸)结合,也能与Gα(q)(GDP)结合,且后一种结合具有不同的蛋白质-蛋白质取向。在细胞中,对荧光标记蛋白的图像分析表明,Gα(q)几乎完全定位于质膜,而PLCβ1在胞质中有相当数量。通过荧光共振能量转移,我们发现在PC12和HEK293细胞中,这些蛋白在未受刺激状态下预先结合在一起。通过测定转染细胞与未转染细胞中这两种蛋白的细胞水平,我们发现在我们的条件下,过表达不应显著促进复合物形成。在单细胞测量和大量(即10^6)细胞悬液测量中均观察到Gα(q)-PLCβ1复合物。考虑到Gα(q)的表达水平高于PLCβ1,且并非所有PLCβ1都定位于质膜,高达约40%(最大值)的高能量共振转移水平令人惊讶。我们的测量结果提示了一种模型,即G蛋白和效应器在激活之前可以以稳定的复合物形式存在,激活是通过分子间相互作用的改变而非扩散和结合来实现的。这些预先形成的复合物进而产生快速、局部的信号。

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