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钙浓度升高可使 NHERF2 和 NHE3 蛋白在负鼠肾(OK)细胞微绒毛中的动态相互作用增强。

Elevated calcium acutely regulates dynamic interactions of NHERF2 and NHE3 proteins in opossum kidney (OK) cell microvilli.

机构信息

Department of Medicine, The Johns Hopkins University School of Medicine, Baltimore, Maryland 21205, USA.

出版信息

J Biol Chem. 2011 Oct 7;286(40):34486-96. doi: 10.1074/jbc.M111.230219. Epub 2011 Jul 28.

Abstract

The brush border (BB) Na(+)/H(+) exchanger NHE3 is rapidly activated or inhibited by changes in trafficking, which mimics renal and intestinal physiology. However, there is a paradox in that NHE3 has limited mobility in the BB due to its binding to the multi-PDZ domain containing the NHERF family. To allow increased endocytosis, as occurs with elevated intracellular Ca(2+), we hypothesized that NHE3 had to be, at least transiently, released from the BB cytoskeleton. Because NHERF1 and -2 are localized at the BB, where they bind NHE3 as well as the cytoskeleton, we tested whether either or both might dynamically interact with NHE3 as part of Ca(2+) signaling. We employed FRET to study close association of NHE3 and these NHERFs and fluorescence recovery after photobleaching to monitor NHE3 mobility in the apical domain in polarized opossum kidney cells. Under basal conditions, NHERF2 and NHE3 exhibited robust FRET signaling. Within 1 min of A23187 (0.5 μm) exposure, the NHERF2-NHE3 FRET signal was abolished, and BB NHE3 mobility was transiently increased. The dynamics in FRET signal and NHE3 mobility correlated well with a change in co-precipitation of NHE3 and NHERF2 but not NHERF1. We conclude the following. 1) Under basal conditions, NHE3 closely associates with NHERF2 in opossum kidney cell microvilli. 2) Within 1 min of elevated Ca(2+), the close association of NHE3-NHERF2 is abolished but is re-established in ∼60 min. 3) The change in NHE3-NHERF2 association is accompanied by an increased BB mobile fraction of NHE3, which contributes to inhibition of NHE3 transport activity via increased endocytosis.

摘要

刷状缘 (BB) Na(+)/H(+) 交换器 NHE3 的转运可迅速被激活或抑制,这模拟了肾脏和肠道的生理功能。然而,存在一个悖论,即由于 NHE3 与包含 NHERF 家族的多 PDZ 结构域结合,因此在 BB 中其移动性有限。为了允许增加内吞作用,如细胞内 Ca(2+) 升高时发生的那样,我们假设 NHE3 必须至少暂时从 BB 细胞骨架中释放出来。由于 NHERF1 和 -2 位于 BB 处,在那里它们与 NHE3 以及细胞骨架结合,我们测试了它们中的一个或两个是否可能作为 Ca(2+) 信号的一部分动态地与 NHE3 相互作用。我们采用 FRET 研究 NHE3 与这些 NHERF 的紧密关联,并采用荧光恢复后漂白来监测极化的负鼠肾细胞中顶域中 NHE3 的流动性。在基础条件下,NHERF2 和 NHE3 表现出强烈的 FRET 信号。在 A23187(0.5μm)暴露后 1 分钟内,NHERF2-NHE3 FRET 信号被消除,并且 BB NHE3 流动性暂时增加。FRET 信号和 NHE3 流动性的动态变化与 NHE3 和 NHERF2 的共沉淀变化很好地相关,但与 NHERF1 无关。我们得出以下结论。1)在基础条件下,NHE3 在负鼠肾细胞微绒毛中与 NHERF2 密切相关。2)在 Ca(2+) 升高后 1 分钟内,NHE3-NHERF2 的紧密关联被消除,但在约 60 分钟后重新建立。3)NHE3-NHERF2 关联的变化伴随着 BB 中 NHE3 的可移动分数增加,这通过增加内吞作用来抑制 NHE3 转运活性。

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