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致密斑细胞对管状液流的直接感知作用。

Direct demonstration of tubular fluid flow sensing by macula densa cells.

机构信息

Zilkha Neurogenetic Institute, ZNI335, Univ. of Southern California, 1501 San Pablo St., Los Angeles, CA 90033, USA.

出版信息

Am J Physiol Renal Physiol. 2010 Nov;299(5):F1087-93. doi: 10.1152/ajprenal.00469.2009. Epub 2010 Aug 18.

Abstract

Macula densa (MD) cells in the cortical thick ascending limb (cTAL) detect variations in tubular fluid composition and transmit signals to the afferent arteriole (AA) that control glomerular filtration rate [tubuloglomerular feedback (TGF)]. Increases in tubular salt at the MD that normally parallel elevations in tubular fluid flow rate are well accepted as the trigger of TGF. The present study aimed to test whether MD cells can detect variations in tubular fluid flow rate per se. Calcium imaging of the in vitro microperfused isolated JGA-glomerulus complex dissected from mice was performed using fluo-4 and fluorescence microscopy. Increasing cTAL flow from 2 to 20 nl/min (80 mM [NaCl]) rapidly produced significant elevations in cytosolic Ca(2+) concentration (Ca(2+)) in AA smooth muscle cells [evidenced by changes in fluo-4 intensity (F); F/F(0) = 1.45 ± 0.11] and AA vasoconstriction. Complete removal of the cTAL around the MD plaque and application of laminar flow through a perfusion pipette directly to the MD apical surface essentially produced the same results even when low (10 mM) or zero NaCl solutions were used. Acetylated α-tubulin immunohistochemistry identified the presence of primary cilia in mouse MD cells. Under no flow conditions, bending MD cilia directly with a micropipette rapidly caused significant Ca(2+) elevations in AA smooth muscle cells (fluo-4 F/F(0): 1.60 ± 0.12) and vasoconstriction. P2 receptor blockade with suramin significantly reduced the flow-induced TGF, whereas scavenging superoxide with tempol did not. In conclusion, MD cells are equipped with a tubular flow-sensing mechanism that may contribute to MD cell function and TGF.

摘要

致密斑(MD)细胞位于皮质升支粗段(cTAL)中,可检测到管状液成分的变化,并将信号传递到入球小动脉(AA),从而控制肾小球滤过率[管球反馈(TGF)]。在 MD 处,通常与管状液流速升高相平行的管状盐浓度增加被认为是 TGF 的触发因素。本研究旨在测试 MD 细胞是否可以检测到管状液流速本身的变化。使用 fluo-4 和荧光显微镜对从小鼠分离的体外微灌注的 JGA-肾小球复合体进行钙成像。将 cTAL 流量从 2 增加到 20 nl/min(80 mM [NaCl])会迅速导致 AA 平滑肌细胞中的细胞内 Ca(2+)浓度 (Ca(2+))显著升高[通过 fluo-4 强度(F)的变化证明;F/F(0) = 1.45 ± 0.11]和 AA 血管收缩。即使使用低(10 mM)或零 NaCl 溶液,完全去除 MD 斑块周围的 cTAL 并通过灌注管直接向 MD 顶端表面施加层流也会产生相同的结果。乙酰化α-微管蛋白免疫组织化学鉴定了小鼠 MD 细胞中初级纤毛的存在。在无流条件下,用微管直接弯曲 MD 纤毛会迅速导致 AA 平滑肌细胞中发生显著的Ca(2+)升高(fluo-4 F/F(0):1.60 ± 0.12)和血管收缩。苏拉明对 P2 受体的阻断显著降低了流量诱导的 TGF,而 Tempol 清除超氧化物则没有。总之,MD 细胞配备了一种管状流速感应机制,可能有助于 MD 细胞功能和 TGF。

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