血管紧张素II亚型1和亚型2受体均参与肾小球上皮细胞胞内钙的调节。

R. Sharma, M. Sharma, S. Vamos, V. Savin, T. Wiegmann
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引用次数: 18

摘要

我们已经证明血管紧张素II (ANG II)的两种受体(AT1和AT2)都参与了肾小球上皮细胞(GECs)细胞内信号的调节。我们研究了这些受体在gec细胞内离子钙[Ca2(+)]i调控中的作用。细胞被加载了Indo-1 (Ca2(+))和SNARF-1 (pH)荧光染料,然后在37℃下加或不加ANG II孵育1小时。在一些实验中,加入at(1)和at(2)受体阻滞剂(分别为氯沙坦和PD 12339)。在另外的实验中,细胞与thapsigargin (Tg)和bradykinin (BK)以及ANG II孵育。使用四通道荧光视频显微镜系统实时测量单个细胞中的[Ca2(+)]i。用放射免疫法测定三磷酸肌醇(IP(3))水平。100nmol /L的ANGⅱ可使含钙缓冲液中[Ca2(+)]i增加最多。ANGⅱ对gec细胞内pH值无影响。同时使用氯沙坦和PD 123319可防止ANG II引起的[Ca2(+)]i升高。BK引起[Ca2(+)]i的短暂增加,ANG II显著降低;氯沙坦与PD 123319同时加入可阻止ANG II的作用。ANG II阻止Ca2(+)在细胞内储存的积累。ANG II引起了显著但短暂的IP水平升高(3)。总之,ANG II增加了gec中细胞外/细胞内钙依赖的双向Ca2(+)运输,抑制了BK诱导的Ca2(+)从IP(3)敏感储存的释放,此外,减少了内质网[Ca2(+)]的再填充,因为反复的BK刺激耗尽了。这两种受体亚型在ANG II介导的gec生理反应中似乎都很重要,并可能参与体内肾小球功能的调节。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Both subtype 1 and 2 receptors of angiotensin II participate in regulation of intracellular calcium in glomerular epithelial cells.
We have documented that both receptors of angiotensin II (ANG II) (AT1 and AT2) are involved in regulation of intracellular signals in glomerular epithelial cells (GECs). We studied the role of these receptors in regulation of intracellular ionized calcium [Ca2(+)]i in GECs. Cells were loaded with Indo-1 (Ca2(+)) and SNARF-1 (pH) fluorescent dyes and then incubated with or without ANG II for 1 hour at 37 degrees C. In some experiments AT(1) and AT(2) receptor blockers (Losartan and PD 12339, respectively) were added. In additional experiments cells were incubated with thapsigargin (Tg) and bradykinin (BK) as well as ANG II. A four-channel fluorescence videomicroscope system was used to measure real-time [Ca2(+) ]i in individual cells. Levels of inositol triphosphate (IP(3)) were measured with radioimmunoassay. An amount of 100 nmol/L of ANG II caused a maximal increase in [Ca2(+)]i in calcium-containing buffer. ANG II had no effect on intracellular pH of GECs. Increase in [Ca2(+)]i by ANG II was prevented by the concurrent use of Losartan and PD 123319. BK caused a transient increase in [Ca2(+)]i, which was significantly decreased by ANG II; concurrent addition of Losartan and PD 123319 prevented ANG II effect. ANG II prevented the accumulation of Ca2(+) in intracellular stores. ANG II caused a significant but transient increase in levels of IP(3). In summary, ANG II increases extracellular/intracellular calcium dependent bidirectional Ca2(+) transport in GECs, inhibits BK induced release of Ca2(+) from IP(3) sensitive stores, and, in addition, reduces refilling of endoplasmic reticulum [Ca2(+)] depleted by repeated BK stimulation. Both receptor subtypes appear to be important in ANG II mediated physiologic responses of GECs and may participate in modulation of glomerular function in vivo.
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