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细胞内钙离子释放对人膀胱平滑肌收缩的作用。

The contribution of intracellular Ca2+ release to contraction in human bladder smooth muscle.

作者信息

Masters J G, Neal D E, Gillespie J I

机构信息

Department of Surgical Sciences, The School of Surgical and Reproductive Sciences, The Medical School, University of Newcastle upon Tyne.

出版信息

Br J Pharmacol. 1999 Jun;127(4):996-1002. doi: 10.1038/sj.bjp.0702640.

Abstract
  1. The importance of Ca2+ release from the sarcoplasmic reticulum (SR) in excitation contraction (EC) coupling in human detrusor muscle remains controversial. In this paper the contribution of Ca2+ release to agonist induced contraction is assessed. 2. Dose response curves to carbachol (0.01 - 10 microM) were constructed before and after exposure to 200 nM Thapsigargin (Tg). Tg pre-treatment reduced the force of contraction at all agonist concentrations however, the reduction was dose dependent. At 0.1 microM the contractions were reduced to 14.5 +/- 7% (mean +/- s.e.mean) of controls (n = 8) while at 10 microM the contractions were only reduced to 92 +/- 3% of controls (n = 10). 3. The role of external Ca2+ was examined by measuring the magnitude of contraction to low and high doses of agonist in the presence and absence of external Ca2+. With (0.1-0.3 microM) carbachol the contractions in nominally Ca2+ free media were 4+/-4% of controls (n = 7) whilst with (1 - 10 microM) carbachol the contractions were 36 +/- 8% of controls (n=7) suggesting that at low agonist concentrations the release of Ca2+ has a requirement for external Ca2+. 4. Pre-treatment of muscle strips with the Ca2+ channel blocking agent diltiazem reduced the contractile responses to carbachol. Contractions induced by 0.1 microM were reduced to 29+/-11% (P<0.05) of controls while those activated by 10 microM were reduced to 86+/-6% (P= 0.1) of controls (n = 4) suggesting the Ca2+ influx needed to activate internal store release at low agonist stimulation is through L-type Ca2+ channels. 5. These observations confirm the importance of thapsigargin sensitive intracellular Ca2+ store release in the activation of contraction of detrusor smooth muscle and suggest the overall contribution of this store depends upon the magnitude of the agonist stimulation.
摘要
  1. 肌浆网(SR)释放Ca2+在人逼尿肌兴奋收缩(EC)偶联中的重要性仍存在争议。本文评估了Ca2+释放在激动剂诱导收缩中的作用。2. 在暴露于200 nM毒胡萝卜素(Tg)之前和之后,构建了对卡巴胆碱(0.01 - 10 microM)的剂量反应曲线。Tg预处理降低了所有激动剂浓度下的收缩力,然而,这种降低是剂量依赖性的。在0.1 microM时,收缩力降低至对照的14.5 +/- 7%(平均值 +/- 标准误平均值)(n = 8),而在10 microM时,收缩力仅降低至对照的92 +/- 3%(n = 10)。3. 通过测量在有无细胞外Ca2+存在的情况下对低剂量和高剂量激动剂的收缩幅度,研究了细胞外Ca2+的作用。使用(0.1 - 0.3 microM)卡巴胆碱时,在名义上无Ca2+的培养基中的收缩力为对照的4 +/- 4%(n = 7),而使用(1 - 10 microM)卡巴胆碱时,收缩力为对照的36 +/- 8%(n = 7),这表明在低激动剂浓度下,Ca2+的释放需要细胞外Ca2+。4. 用Ca2+通道阻滞剂地尔硫卓预处理肌条可降低对卡巴胆碱的收缩反应。由0.1 microM诱导的收缩力降低至对照的29 +/- 11%(P < 0.05),而由10 microM激活的收缩力降低至对照的86 +/- 6%(P = 0.1)(n = 4),这表明在低激动剂刺激下激活内部储存释放所需的Ca2+内流是通过L型Ca2+通道。5. 这些观察结果证实了毒胡萝卜素敏感的细胞内Ca2+储存释放在逼尿肌平滑肌收缩激活中的重要性,并表明该储存的总体贡献取决于激动剂刺激的幅度。

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