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成年和新生大鼠颌下唾液腺细胞中的钙离子动员和氯离子外流

Ca2+ mobilization and Cl efflux in submandibular salivary cells of adult and newborn rats.

作者信息

Martinez J R, Camden J

机构信息

Department of Child Health, University of Missouri School of Medicine, Columbia 65212.

出版信息

Arch Oral Biol. 1989;34(3):147-52. doi: 10.1016/0003-9969(89)90001-0.

Abstract

These cells were isolated by enzymatic digestion from glands of 1-day-old and fully mature rats. The effects of exposure to acetylcholine on cytosolic Ca2+ and Cl efflux were studied by, respectively, spectrofluorimetry of fura-2 and the net efflux of the isotopic tracer 36Cl from preloaded cells. In both types of cells, when incubated in Ca2+-containing solutions, acetylcholine initially caused a rapid, significant increase in cytosolic Ca2+ (from approx. 90 to 480-570 nmol), followed by a slower decrease to a plateau value of 280-290 nmol. The initial peak persisted (315-339 nmol) in Ca2+-free solutions but the cytosolic Ca2+ concentrations decreased rapidly to levels below prestimulation values (30 nmol). 36Cl efflux in tracer preloaded cells incubated in Ca2+-containing medium in the presence of acetylcholine was 18% in cells of new born animals and 35% in adult cells. In Ca2+-free medium, mature cells showed a transient but significant (26%) efflux of 36Cl. Cells of 1-day-old rats did not show a net efflux of 36Cl under these conditions, but subsequent addition of Ca2+ caused a 15% reduction (i.e. efflux) in tracer content. The antagonist 3,4,5-trimethoxybenzoate-8(N,N-dithylamino)octyl ester (TMB 8), which blocks internal Ca2+ release, inhibited both the initial increase in cell Ca2+ in both types of cells and the transient efflux of 36Cl seen in mature cells when incubated in Ca2+-free solutions. At high concentrations (5 mM), LaCl3 inhibited efflux of 36Cl in mature cells but not in those of newborn rats. However, at lower concentrations (0.1 mM), which do not interfere with fluorescence spectra, LaCl3 did not inhibit the effect of acetylcholine on cell Ca2+. These results suggest that Cl efflux in adult submandibular cells is regulated by an increase in cell Ca2+ arising from release of internal Ca2+ and from influx of external Ca2+. Both of these responses are evident in cells of newborn animals but Cl efflux is either decreased or absent. This is likely to be associated with a deficiency in the Cl channels or in the coupling between Ca2+ and the channel substrate through regulatory molecules associated with phosphorylation of the channel protein.

摘要

这些细胞是通过酶消化法从1日龄和完全成熟大鼠的腺体中分离出来的。分别采用fura-2荧光分光光度法和预加载细胞中同位素示踪剂36Cl的净流出量研究了乙酰胆碱暴露对细胞质Ca2+和Cl流出的影响。在这两种类型的细胞中,当在含Ca2+的溶液中孵育时,乙酰胆碱最初会导致细胞质Ca2+迅速显著增加(从约90增加到480 - 570 nmol),随后缓慢下降至280 - 290 nmol的平台值。在无Ca2+溶液中,初始峰值持续存在(315 - 339 nmol),但细胞质Ca2+浓度迅速降至低于刺激前值(30 nmol)的水平。在含乙酰胆碱的含Ca2+培养基中孵育的预加载示踪剂细胞中,新生动物细胞的36Cl流出量为18%,成年细胞为35%。在无Ca2+培养基中,成熟细胞显示出短暂但显著的(26%)36Cl流出。在这些条件下,1日龄大鼠的细胞未显示出36Cl的净流出,但随后添加Ca2+导致示踪剂含量减少15%(即流出)。阻断细胞内Ca2+释放的拮抗剂3,4,5 - 三甲氧基苯甲酸 - 8(N,N - 二乙氨基)辛酯(TMB 8),抑制了两种类型细胞中细胞Ca2+的初始增加以及在无Ca2+溶液中孵育时成熟细胞中观察到的36Cl的短暂流出。在高浓度(5 mM)时,LaCl3抑制成熟细胞中36Cl的流出,但不抑制新生大鼠细胞中的流出。然而,在不干扰荧光光谱的较低浓度(0.1 mM)下,LaCl3不抑制乙酰胆碱对细胞Ca2+的作用。这些结果表明,成年下颌下腺细胞中的Cl流出受细胞内Ca2+释放和细胞外Ca2+流入引起的细胞Ca2+增加的调节。这两种反应在新生动物细胞中都很明显,但Cl流出要么减少要么不存在。这可能与Cl通道的缺陷或通过与通道蛋白磷酸化相关的调节分子在Ca2+与通道底物之间的偶联缺陷有关。

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