Soltoff S P, McMillian M K, Cragoe E J, Cantley L C, Talamo B R
Department of Physiology, Tufts University, Boston, Massachusetts 02111.
J Gen Physiol. 1990 Feb;95(2):319-46. doi: 10.1085/jgp.95.2.319.
The effects of extracellular ATP on ion fluxes and the intracellular free Ca2+ concentration ([Ca2+]i) were examined using a suspension of rat parotid acinar cells and were contrasted with the effects of the muscarinic agonist carbachol. Although ATP and carbachol both rapidly increased [Ca2+]i about threefold above the resting level (200-250 nM), the effect of ATP was due primarily to an influx of Ca2+ across the plasma membrane, while the initial response to carbachol was due to a release of Ca2+ from intracellular stores. Within 10 s, ATP (1 mM) and carbachol (20 microM) reduced the cellular Cl- content by 39-50% and cell volume by 15-25%. Both stimuli reduced the cytosolic K+ content by 57-65%, but there were marked differences in the rate and pattern of net K+ movement as well as the effects of K+ channel inhibitors on the effluxes initiated by the two stimuli. The maximum rate of the ATP-stimulated K+ efflux (approximately 2,200 nmol K+/mg protein per min) was about two-thirds that of the carbachol-initiated efflux rate, and was reduced by approximately 30% (vs. 60% for the carbachol-stimulated K+ efflux) by TEA (tetraethylammonium), an inhibitor of the large conductance (BK) K+ channel. Charybdotoxin, another K+ channel blocker, was markedly more effective than TEA on the effects of both agonists, and reduced the rate of K+ efflux initiated by both ATP and carbachol by approximately 80%. The removal of extracellular Ca2+ reduced the ATP- and the carbachol-stimulated rates of K+ efflux by 55 and 17%, respectively. The rate of K+ efflux initiated by either agonist was reduced by 78-95% in cells that were loaded with BAPTA to slow the elevation of [Ca2+]i. These results indicated that ATP and carbachol stimulated the efflux of K+ through multiple types of K(+)-permeable channels, and demonstrated that the relative proportion of efflux through the different pathways was different for the two stimuli. ATP and carbachol also stimulated the rapid entry of Na+ into the parotid cell, and elevated the intracellular Na+ content to 4.4 and 2.6 times the normal level, respectively. The rate of Na+ entry through Na(+)-K(+)-2Cl- cotransport and Na(+)-H+ exchange was similar whether stimulated by ATP, carbachol, or ionomycin, and uptake through these two carrier-mediated transporters accounted for 50% of the ATP-promoted Na+ influx. The remainder may be due to a nonselective cation channel and an ATP-gated cation channel that is also permeable to Ca2+.(ABSTRACT TRUNCATED AT 400 WORDS)
利用大鼠腮腺腺泡细胞悬液研究了细胞外ATP对离子通量和细胞内游离Ca2+浓度([Ca2+]i)的影响,并与毒蕈碱激动剂卡巴胆碱的作用进行了对比。尽管ATP和卡巴胆碱均可使[Ca2+]i迅速升高至静息水平(200 - 250 nM)以上约三倍,但ATP的作用主要是由于Ca2+跨质膜内流,而对卡巴胆碱的初始反应则是由于细胞内储存的Ca2+释放。在10秒内,ATP(1 mM)和卡巴胆碱(20 μM)使细胞Cl-含量降低了39 - 50%,细胞体积减少了15 - 25%。两种刺激均使胞质K+含量降低了57 - 65%,但在净K+移动的速率和模式以及K+通道抑制剂对两种刺激引发的外流的影响方面存在显著差异。ATP刺激的K+外流的最大速率(约2200 nmol K+/mg蛋白每分钟)约为卡巴胆碱引发的外流速率的三分之二,并且被大电导(BK)K+通道抑制剂TEA(四乙铵)降低了约30%(而卡巴胆碱刺激的K+外流降低了60%)。另一种K+通道阻滞剂蝎毒素对两种激动剂的作用明显比TEA更有效,并使ATP和卡巴胆碱引发的K+外流速率降低了约80%。去除细胞外Ca2+分别使ATP和卡巴胆碱刺激的K+外流速率降低了55%和17%。在加载了BAPTA以减缓[Ca2+]i升高的细胞中,由任一激动剂引发的K+外流速率降低了78 - 95%。这些结果表明,ATP和卡巴胆碱通过多种类型的K+渗透通道刺激K+外流,并表明两种刺激通过不同途径外流的相对比例不同。ATP和卡巴胆碱还刺激Na+迅速进入腮腺细胞,并使细胞内Na+含量分别升高至正常水平的4.4倍和2.6倍。无论是由ATP、卡巴胆碱还是离子霉素刺激,通过Na+-K+-2Cl-共转运和Na+-H+交换的Na+进入速率相似,通过这两种载体介导的转运体的摄取占ATP促进的Na+内流的50%。其余部分可能归因于一种非选择性阳离子通道和一种也可通透Ca2+的ATP门控阳离子通道。(摘要截短至400字)
