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首页> 外文期刊>American Journal of Physiology >Effects of luminal flow and nucleotides on (Ca(2+))(i) in rabbit cortical collecting duct.
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Effects of luminal flow and nucleotides on (Ca(2+))(i) in rabbit cortical collecting duct.

机译:腔流量和核苷酸对兔皮质收集管中(Ca(2 +))(i)的影响。

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摘要

Nucleotide binding to purinergic P2 receptors contributes to the regulation of a variety of physiological functions in renal epithelial cells. Whereas P2 receptors have been functionally identified at the basolateral membrane of the cortical collecting duct (CCD), a final regulatory site of urinary Na(+), K(+), and acid-base excretion, controversy exists as to whether apical purinoceptors exist in this segment. Nor has the distribution of receptor subtypes present on the unique cell populations that constitute Ca(2+) the CCD been established. To examine this, we measured nucleotide-induced changes in intracellular Ca(2+) concentration ([Ca(2+)](i)) in fura 2-loaded rabbit CCDs microperfused in vitro. Resting [Ca(2+)](i) did not differ between principal and intercalated cells, averaging approximately 120 nM. An acute increase in tubular fluid flow rate, associated with a 20% increase in tubular diameter, led to increases in [Ca(2+)](i) in both cell types. Luminal perfusion of 100 microM UTP or ATP-gamma-S, in the absence of change in flow rate, caused a rapid and transient approximately fourfold increase in [Ca(2+)](i) in both cell types (P < 0.05). Luminal suramin, a nonspecific P2 receptor antagonist, blocked the nucleotide- but not flow-induced [Ca(2+)](i) transients. Luminal perfusion with a P2X (alpha,beta-methylene-ATP), P2X(7) (benzoyl-benzoyl-ATP), P2Y(1) (2-methylthio-ATP), or P2Y(4)/P2Y(6) (UDP) receptor agonist had no effect on [Ca(2+)](i). The nucleotide-induced [Ca(2+)](i) transients were inhibited by the inositol-1,4,5-triphosphate receptor blocker 2-aminoethoxydiphenyl borate, thapsigargin, which depletes internal Ca(2+) stores, luminal perfusion with a Ca(2+)-free perfusate, or the L-type Ca(2+) channel blocker nifedipine. These results suggest that luminal nucleotides activate apical P2Y(2) receptors in the CCD via pathways that require both internal Ca(2+) mobilization and extracellular Ca(2+) entry. The flow-induced rise in [Ca(2+)](i) is apparently not mediated by apical P2 purinergic receptor signaling.
机译:与嘌呤能P2受体结合的核苷酸有助于调节肾上皮细胞的多种生理功能。 P2受体已在皮层收集管(CCD)的基底外侧膜,尿中Na(+),K(+)和酸碱排泄的最终调节位点上进行了功能鉴定,但关于是否存在根尖型嘌呤受体存在争议在这个细分市场中也没有建立组成CCD的Ca(2+)的独特细胞群上存在的受体亚型的分布。若要检查这一点,我们测量了呋喃2加载兔CCD体外灌注的核苷酸诱导的细胞内Ca(2+)浓度([Ca(2 +)](i))的变化。静止的[Ca(2 +)](i)在主细胞和插入细胞之间没有差异,平均大约为120 nM。管状液体流速的急剧增加,与管状直径增加20%相关,导致两种细胞类型中[Ca(2 +)](i)的增加。在没有流速变化的情况下,对100 microM UTP或ATP-γ-S进行光灌注,导致两种细胞类型中[Ca(2 +)](i)的快速和瞬时增加大约四倍(P <0.05) 。 Luminal suramin,一种非特异性的P2受体拮抗剂,阻断了核苷酸,但未阻断血流诱导的[Ca(2 +)](i)瞬变。 P2X(α,β-亚甲基-ATP),P2X(7)(苯甲酰基-苯甲酰基-ATP),P2Y(1)(2-甲硫基-ATP)或P2Y(4)/ P2Y(6)的光灌注UDP)受体激动剂对[Ca(2 +)](i)没有影响。核苷酸诱导的[Ca(2 +)](i)瞬变被肌醇-1,4,5-三磷酸受体阻滞剂2-氨基乙氧基二苯基硼酸盐thapsigargin抑制,从而耗尽了内部Ca(2+)存储,腔内灌注无Ca(2+)灌注液或L型Ca(2+)通道阻滞剂硝苯地平。这些结果表明,腔核苷酸通过需要内部Ca(2+)动员和细胞外Ca(2+)进入的途径激活CCD中的顶P2Y(2)受体。流量诱导的[Ca(2 +)](i)升高显然不是由顶端P2嘌呤能受体信号传导介导的。

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