首页> 美国卫生研究院文献>The Journal of Physiology >Focal Ca2+i increases detected by aequorin but not by fura-2 in histamine- and caffeine-stimulated swine carotid artery.
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Focal Ca2+i increases detected by aequorin but not by fura-2 in histamine- and caffeine-stimulated swine carotid artery.

机译:在组胺和咖啡因刺激的猪颈动脉中水母发光蛋白检测到的局部Ca2 + i升高而呋喃2检测不到。

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摘要

1. We hypothesized that the homogeneity of intracellular [Ca2+] ([Ca2+]i) varies and is regulated in arterial smooth muscle. 2. We evaluated this hypothesis by exploiting the different characteristics of several [Ca2+]i indicators: (1) aequorin, which theoretically can measure focal increases in [Ca2+]i, (2) fura-2, which is predominantly a measure of mean cytoplasmic [Ca2+], and (3) myosin light chain phosphorylation and force, which reflect increases in [Ca2+] near the contractile apparatus. 3. From the differences in the observed aequorin and fura-2 signals, we developed an index of the relative degree of [Ca2+]i homogeneity as the ratio of the aequorin signal and fura-2 signal. 4. Stimulation with intermediate concentrations of histamine (1 and 10 microM) or high [K+]o (25 and 40 mM) increased [Ca2+]i and contractile stress. Relative [Ca2+]i homogeneity, estimated from the aequorin/fura-2 ratio, remained similar to levels observed in unstimulated tissues. 5. Higher concentrations of histamine (100 microM) also increased [Ca2+]i and stress, but the aequorin/fura 2 ratio declined , indicating increased [Ca2+]i homogeneity. Similarly, the aequorin/fura-2 ratio decreased when extracellular Ca2+ was removed. 6. Stimulation with histamine in low extracellular [Ca2+] transiently increased [Ca2+]i and the aequorin/fura-2 ratio. Similarly, in tissues treated with low extracellular [Ca2+], restoration of extracellular Ca2+ transiently increased both [Ca2+]i and the aequorin/fura-2 ratio. Although both of these experiments demonstrated a transient decrease in [Ca2+]i homogeneity, only histamine stimulation led to increased myosin light chain phosphorylation and force. These results indicate that the focal increases in [Ca2+]i observed with histamine stimulation and Ca2+ restoration occurred in different cellular regions. 7. Addition of caffeine (20 mM) increased [Ca2+]i and [cAMP], but this was not accompanied by sustained increased myosin light chain phosphorylation or contraction. Phosphorylation of myosin light chain kinase did not appear to underlie the lack of increase in myosin light chain phosphorylation. Rather, caffeine induced a sustained increase in the aequorin/fura-2 ratio, suggesting that caffeine inhibits smooth muscle contraction by localizing increases in [Ca2+]i to a region distant from the contractile apparatus. 8. These data suggest that there can be transient and sustained focal increases in [Ca2+]i. Aequorin detected increased [Ca2+]i in small regions of the cytoplasm during release from and refilling of the intracellular Ca2+ store and with caffeine stimulation. Dual use of aequorin and fura-2 permits determination of relative [Ca2+]i homogeneity in smooth muscle.
机译:1.我们假设细胞内[Ca2 +]([Ca2 +] i)的均一性在动脉平滑肌中发生变化并受到调节。 2.我们通过利用几个[Ca2 +] i指标的不同特征评估了这一假设:(1)水母发光蛋白,理论上可以测量[Ca2 +] i的病灶增加,(2)fura-2,主要是平均值的量度胞质[Ca2 +]和(3)肌球蛋白轻链的磷酸化和作用力,反映了收缩装置附近[Ca2 +]的增加。 3.根据所观察到的水母发光蛋白和fura-2信号的差异,我们开发了[Ca2 +] i同质性相对程度的指标,即水母发光蛋白信号和fura-2信号的比率。 4.用中等浓度的组胺(1和10 microM)或高[K +] o(25和40 mM)刺激会增加[Ca2 +] i和收缩应激。根据水母发光蛋白/ fura-2比率估算的相对[Ca2 +] i同质性,与未刺激组织中观察到的水平相似。 5.较高浓度的组胺(100 microM)也增加了[Ca2 +] i和胁迫,但水母发光蛋白/富拉2的比率下降,表明[Ca2 +] i均一性增加。同样,当去除细胞外Ca2 +时,水母发光蛋白/ fura-2比率降低。 6.在低细胞外[Ca2 +]中用组胺刺激会瞬时增加[Ca2 +] i和水母发光蛋白/ fura-2的比率。同样,在低细胞外[Ca2 +]处理的组织中,细胞外Ca2 +的恢复会瞬时增加[Ca2 +] i和水母发光蛋白/ fura-2的比率。尽管这两个实验都证明[Ca2 +] i均一性暂时降低,但仅组胺刺激会导致肌球蛋白轻链磷酸化和作用力增加。这些结果表明,通过组胺刺激观察到的[Ca2 +] i的局灶性增加和Ca2 +的恢复发生在不同的细胞区域。 7.添加咖啡因(20 mM)可增加[Ca2 +] i和[cAMP],但这并没有伴随着肌球蛋白轻链磷酸化或收缩的持续增加。肌球蛋白轻链激酶的磷酸化似乎没有表明缺乏肌球蛋白轻链磷酸化的增加。而是,咖啡因诱导了水母发光蛋白/ fura-2比值的持续增加,这表明咖啡因通过将[Ca2 +] i的增加局限在远离收缩装置的区域来抑制平滑肌收缩。 8.这些数据表明[Ca2 +] i可能有短暂的和持续的局灶性增加。在释放和补充细胞内Ca2 +储存并补充咖啡因的过程中,水母发光蛋白在细胞质小区域检测到[Ca2 +] i升高。水母发光蛋白和呋喃2的双重使用可以确定平滑肌中[Ca2 +] i的相对同质性。

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