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前列腺素F2α可在通过缝隙连接耦合的NRK成纤维细胞单层中诱导非同步的细胞内钙振荡。

Prostaglandin F2 alpha induces unsynchronized intracellular calcium oscillations in monolayers of gap junctionally coupled NRK fibroblasts.

作者信息

Harks Erik G A, Scheenen Wim J J M, Peters Peter H J, van Zoelen Everardus J J, Theuvenet Alexander P R

机构信息

Department of Cell Biology, University of Nijmegen, Toernooiveld 1, 6525 ED Nijmegen, The Netherlands.

出版信息

Pflugers Arch. 2003 Oct;447(1):78-86. doi: 10.1007/s00424-003-1126-8. Epub 2003 Jul 8.

Abstract

We investigated the intracellular calcium oscillations induced by prostaglandin F2alpha (PGF2alpha) in individual cells of confluent, gap junction-coupled monolayers of normal rat kidney (NRK) fibroblasts. PGF2alpha (1000 nM) induced oscillations in more than 90% of the cells in the monolayer, but the frequency of these oscillations was highly variable between individual cells (0.2-1.4 min(-1)). The initial calcium peak resulted from calcium release from IP3-sensitive stores, while subsequent calcium transients were mediated by interplay between both IP3-sensitive calcium stores and calcium influx. The oscillation frequency was increased by sensitizing the IP3 receptor with thimerosal (10 microM) and depended on the extracellular calcium concentration. Thapsigargin (5 nM), which inhibits reuptake of calcium into the stores, only seemed to reduce the amplitude of the oscillation. Patch-clamp experiments revealed that PGF2alpha did not inhibit electrical coupling of the NRK cells in the monolayer. Gap junctional permeability of NRK cells thus appears to be sufficient to allow electrical coupling, resulting in a uniform membrane potential throughout the entire monolayer, but insufficient to synchronize the intracellular calcium oscillations upon PGF2alpha stimulation.

摘要

我们研究了前列腺素F2α(PGF2α)在正常大鼠肾(NRK)成纤维细胞汇合的、通过缝隙连接耦合的单层细胞中诱导的细胞内钙振荡。PGF2α(1000 nM)在单层中90%以上的细胞中诱导了振荡,但这些振荡的频率在单个细胞之间高度可变(0.2 - 1.4 min⁻¹)。最初的钙峰源于IP3敏感储存库中的钙释放,而随后的钙瞬变是由IP3敏感钙储存库和钙内流之间的相互作用介导的。通过用硫柳汞(10 μM)使IP3受体敏感化可增加振荡频率,且振荡频率取决于细胞外钙浓度。毒胡萝卜素(5 nM)可抑制钙重新摄取到储存库中,它似乎仅降低了振荡的幅度。膜片钳实验表明,PGF2α不抑制单层中NRK细胞的电耦合。因此,NRK细胞的缝隙连接通透性似乎足以实现电耦合,导致整个单层具有均匀的膜电位,但在PGF2α刺激时不足以使细胞内钙振荡同步。

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