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Characteristics of the bradykinin-induced changes in intracellular calcium ion concentration of single bovine tracheal smooth muscle cells

机译:缓激肽诱导的牛气管平滑肌细胞内钙离子浓度变化的特征

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摘要

1Single bovine tracheal smooth muscle (BTSM) cells were cultured and used to measure bradykinin-induced changes in [Ca2+]i by dynamic video imaging.\ud2Bradykinin (10 pm-10 μm)-induced an increase in [Ca2+]i over basal levels (69 ± 2 nm; n = 353) which was concentration-dependent (log EC50 = −8.7 m) in the presence of extracellular calcium ions (2 mm). The bradykinin B2 receptor antagonist, d-Arg[Hyp3,Thi5,8,d-Phe7]-bradykinin, produced a parallel shift to the right of the bradykinin concentration-response curve (log EC50 = −7.1 m and −5.8 m in the presence of 1 μm and 10 μm antagonist respectively) yielding an apparent KD of 26 nm.\ud3In the absence of extracellular calcium ions (with 0.1 mm EGTA), bradykinin (10 pm– 10 μm) produced a uniform increase in [Ca2+]i from a basal level of 33 ± 2 nm (n = 140) to approximately 180 nm in BTSM cells indicating an ‘all-or-nothing’ release of intracellular calcium ions. In the presence of 10 μm d-Arg[Hyp3,Thi5,8,d-Phe7]-bradykinin no responses could be induced by bradykinin at concentrations below 100 nm. However, at 100 nm and 1 μm bradykinin there was no change in the uniform increase in [Ca2+]i in these cells previously observed.\ud4In both the absence or presence of d-Arg[Hyp3,Thi5,8,d-Phe7]-bradykinin, there was a concentration-dependent increase in the percentage of cells responding to bradykinin (frequency) under calcium-rich or calcium-free conditions. Individual cells also demonstrated a difference in the sensitivity to any particular concentration of bradykinin.\ud5A latency in the response of cells to bradykinin was observed both in calcium-containing and calcium-free conditions.\ud6We conclude that bradykinin B2 receptors are expressed by BTSM cells and are involved in the bradykinin-induced increase in [Ca2+]i. It appears that the increase in [Ca2+]i can be mediated via a graded influx of calcium ions from the extracellular space or an ‘all-or-nothing’ release from intracellular stores.
机译:1培养了单个牛气管平滑肌(BTSM)细胞,并通过动态视频成像测量了缓激肽诱导的[Ca2 +] i变化。\ ud2Bradykinin(10 pm-10μm)诱导了[Ca2 +] i超过基础水平的增加。 (69±2 nm; n = 353)在存在细胞外钙离子(2 mm)时呈浓度依赖性(log EC50 = -8.7 m)。缓激肽B2受体拮抗剂d-Arg [Hyp3,Thi5,8,d-Phe7]-缓激肽在缓激肽浓度-反应曲线的右侧产生了一个平行位移(log EC50 = -7.1 m和-5.8 m在\ ud3在没有1μm和10μm拮抗剂的情况下,其表观KD值约为26 nm。\ ud3在不存在细胞外钙离子(含0.1 mm EGTA)的情况下,缓激肽(10 pm– 10μm)使[Ca2 +] i均匀增加从BTSM细胞的基础水平33±2 nm(n = 140)到大约180 nm,表明细胞内钙离子“全部或全部”释放。在10μmd-Arg [Hyp3,Thi5,8,d-Phe7]-缓激肽的存在下,缓激肽在低于100 nm的浓度下不会诱导任何应答。但是,在100 nm和1μm的缓激肽下,先前观察到的这些细胞中[Ca2 +] i的均匀增加没有变化。\ ud4无论是否存在d-Arg [Hyp3,Thi5,8,d-Phe7] -缓激肽,在富含钙或无钙的条件下,响应缓激肽的细胞百分比(频率)呈浓度依赖性增加。个别细胞还表现出对任何特定浓度的缓激肽敏感性的差异。\ ud5A在含钙和无钙条件下均观察到了细胞对缓激肽反应的潜伏期。\ ud6我们得出结论,缓激肽B2受体由BTSM表达。细胞并参与缓激肽诱导的[Ca2 +] i的增加。看来[Ca2 +] i的增加可以通过细胞外空间钙离子的逐步流入或细胞内存储的“全有或全无”释放来介导。

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