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激动剂和氯苯丙氨酸诱导家兔完整瓣膜内皮细胞质游离钙离子浓度升高。

Agonist- and CPA-induced elevation of cytoplasmic free Ca2+ in intact valvular endothelium from rabbits.

作者信息

Li L, van Breemen C

机构信息

Department of Pharmacology and Therapeutics, University of British Columbia, Faculty of Medicine, Vancouver, Canada.

出版信息

Am J Physiol. 1996 Mar;270(3 Pt 2):H837-48. doi: 10.1152/ajpheart.1996.270.3.H837.

DOI:10.1152/ajpheart.1996.270.3.H837
PMID:8780177
Abstract

Intracellular Ca2+ signals of intact endothelium from rabbit aortic or pulmonic valves loaded with fura 2 were studied using imaging fluorescence microscopy. Agonists such as ATP or carbachol and inhibitors of endoplasmic reticulum (ER) Ca(2+)-ATPase such as cyclopiazonic acid (CPA), thapsigargin, and 2', 5'-di(tert-butyl)-1, 4,-benzohydroquinone (BHQ) induced an increase in cytoplasmic free Ca2+ concentration ([Ca2+]i) that was maintained above the prestimulated levels as long as extracellular Ca2+ was present, indicating that the maintained [Ca2+]i increase is dependent on the entry of extracellular Ca2+. The voltage-gated channel was not found to contribute to [Ca2+]i increase. SK&F-96365, a receptor-operated cation channel (ROC) blocker, and 2-nitro-4-carboxyphenyl-N, N-diphenylcarbamate (NCDC), a postulated phospholipase C inhibitor, were shown to effectively block ROC, since they greatly reduced the maintained [Ca2+]i increase caused by ATP, but not that caused by CPA, which was blocked by Ni2+. To further investigate the Ca2+ influx involved in this process, divalent cation entry was measured as Mn2+ quenching of fura 2 fluorescence at 360-nm excitation wavelength. At rest, fluorescence quenching at 360 nm by Mn2+ was observed, which was inhibited by Ni2+ but not by NCDC, indicating Mn2+ entry through the leak pathway. The quenching was enhanced following ATP stimulation, and this enhancement was abolished by pretreatment with NCDC. In contrast, the rate of Mn2+ quenching was unaffected by the application of CPA. These results demonstrate that ATP stimulates divalent cation influx that is not related to the Ca2+ content of ER. Abolition of Ca2+ uptake into ER was postulated to increase the effectiveness of the Ca2+ leak in raising [Ca2+]i.

摘要

采用成像荧光显微镜研究了用fura 2负载的兔主动脉瓣或肺动脉瓣完整内皮细胞的细胞内Ca2+信号。ATP或卡巴胆碱等激动剂以及内质网(ER)Ca(2+)-ATP酶抑制剂如环匹阿尼酸(CPA)、毒胡萝卜素和2', 5'-二(叔丁基)-1, 4-苯并对苯二酚(BHQ)可诱导细胞质游离Ca2+浓度([Ca2+]i)升高,只要细胞外Ca2+存在,该浓度就维持在刺激前水平之上,这表明[Ca2+]i的持续升高依赖于细胞外Ca2+的内流。未发现电压门控通道对[Ca2+]i升高有贡献。受体操纵性阳离子通道(ROC)阻滞剂SK&F-96365和假定的磷脂酶C抑制剂2-硝基-4-羧基苯基-N, N-二苯基氨基甲酸酯(NCDC)被证明可有效阻断ROC,因为它们大大降低了ATP引起的[Ca2+]i持续升高,但对CPA引起的升高没有影响,CPA引起的升高可被Ni2+阻断。为了进一步研究该过程中涉及的Ca2+内流,在360 nm激发波长下,通过fura 2荧光的Mn2+淬灭来测量二价阳离子内流。静息时,观察到Mn2+在360 nm处的荧光淬灭,该淬灭被Ni2+抑制但不被NCDC抑制,表明Mn2+通过泄漏途径进入。ATP刺激后淬灭增强,且该增强被NCDC预处理消除。相反,CPA的应用不影响Mn2+淬灭速率。这些结果表明,ATP刺激二价阳离子内流,且该内流与内质网的Ca2+含量无关。内质网Ca2+摄取的消除被认为可增加Ca2+泄漏在升高[Ca2+]i方面的有效性。

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