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毒蕈碱诱导的质膜Ca2 + -ATP酶募集涉及PSD-95/Dlg/Zo-1介导的相互作用。

Muscarinic-induced recruitment of plasma membrane Ca2+-ATPase involves PSD-95/Dlg/Zo-1-mediated interactions.

作者信息

Kruger Wade A, Yun C Chris, Monteith Gregory R, Poronnik Philip

机构信息

School of Biomedical Sciences and School of Pharmacy, The University of Queensland, Brisbane QLD 4072, Australia.

出版信息

J Biol Chem. 2009 Jan 16;284(3):1820-30. doi: 10.1074/jbc.M804590200. Epub 2008 Nov 18.

Abstract

Efflux of cytosolic Ca2+ mediated by plasma membrane Ca2+-ATPases (PMCA) plays a key role in fine tuning the magnitude and duration of Ca2+ signaling following activation of G-protein-coupled receptors. However, the molecular mechanisms that underpin the trafficking of PMCA to the membrane during Ca2+ signaling remain largely unexplored in native cell models. One potential mechanism for the recruitment of proteins to the plasma membrane involves PDZ interactions. In this context, we investigated the role of PMCA interactions with the Na+/H+ exchanger regulatory factor 2 (NHERF-2) during muscarinic-induced Ca2+ mobilization in the HT-29 epithelial cell line. GST pull-downs in HT-29 cell lysates showed that the PDZ2 module of NHERF-2 bound to the PDZ binding motif on the C terminus of PMCA. Co-immunoprecipitations confirmed that PMCA1b and NHERF-2 associated under normal conditions in HT-29 cells. Cell surface biotinylations revealed significant increases in membrane-associated NHERF-2 and PMCA within 60 s following muscarinic activation, accompanied by increased association of the two proteins as seen by confocal microscopy. The recruitment of NHERF-2 to the membrane preceded that of PMCA, suggesting that NHERF-2 was involved in nucleating an efflux complex at the membrane. The muscarinic-mediated translocation of PMCA was abolished when NHERF-2 was silenced, and the rate of relative Ca2+ efflux was also reduced. These experiments also uncovered a NHERF-2-independent PMCA retrieval mechanism. Our findings describe rapid agonist-induced translocation of PMCA in a native cell model and suggest that NHERF-2 plays a key role in scaffolding and maintaining PMCA at the cell membrane.

摘要

质膜Ca2+ -ATP酶(PMCA)介导的胞质Ca2+外流在微调G蛋白偶联受体激活后Ca2+信号的强度和持续时间方面起着关键作用。然而,在天然细胞模型中,Ca2+信号传导过程中PMCA转运至细胞膜的分子机制在很大程度上仍未得到探索。蛋白质募集到质膜的一种潜在机制涉及PDZ相互作用。在此背景下,我们研究了在HT - 29上皮细胞系中,毒蕈碱诱导的Ca2+动员过程中PMCA与Na+/H+交换调节因子2(NHERF - 2)相互作用的作用。HT - 29细胞裂解物中的GST下拉实验表明,NHERF - 2的PDZ2模块与PMCA C末端的PDZ结合基序结合。免疫共沉淀证实,在正常条件下HT - 29细胞中PMCA1b和NHERF - 2相互关联。细胞表面生物素化显示,毒蕈碱激活后60秒内,膜相关的NHERF - 2和PMCA显著增加,共聚焦显微镜观察到这两种蛋白质的结合也增加。NHERF - 2募集到膜上先于PMCA,这表明NHERF - 2参与在膜上形成一个外流复合物。当NHERF - 2沉默时,毒蕈碱介导的PMCA易位被消除,相对Ca2+外流速率也降低。这些实验还揭示了一种不依赖NHERF - 2的PMCA回收机制。我们的研究结果描述了在天然细胞模型中激动剂诱导的PMCA快速易位,并表明NHERF - 2在将PMCA支架化并维持在细胞膜上起关键作用。

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