Bkaily G, Jaalouk D, Jacques D, Economos D, Hassan G, Simaan M, Regoli D, Pothier P
Department of Anatomy and Cell Biology, Faculty of Medicine, Université de Sherbrooke, QC, Canada.
Can J Physiol Pharmacol. 1997 Jun;75(6):652-60.
The mechanism(s) fo Ca2+ entry stimulated by bradykinin (BK) and the receptor subtype responsible for this effect were examined in human and rabbit aortic vascular smooth muscle cells (VSMCs). Using the whole-cell voltage clamp technique, BK (10(-6)M) significantly (p < 0.05) increased both T- and L-type Ca2+ currents (ICa) in rabbit aortic VSMCs. Using the fura-2 total intracellular Ca2+ ([Ca]i) measurement technique, BK (10(-6) M) induced a transient increase of [Ca]i followed by a sustained component. Pretreatment of rabbit VSMCs with sarcoplasmic reticulum (SR) Ca2+ releaser caffeine (1-5 mM) significantly decreased the BK-induced transient increase of [Ca]i without affecting the sustained component induced by this hormone. This sustained phase was blocked by extracellular application of the Ca2+ chelator EGTA. Using the fluo-3 confocal microscopy Ca2+ measurement technique to localize cytosolic ([Ca]c) and nuclear ([Ca]n) free Ca2+ distribution, the resting sustained concentration of Ca2+ in the cytoplasm of rabbit and human aortic VSMCs was less than that in the nucleus. BK (10(-7) M) induced a nonsignificant sustained increase of [Ca]c but significant (p < 0.05) sustained increase of [Ca]n that was reversed but not prevented by the specific B1 receptor antagonist R126 (10(-6) M) as well as by the B2 receptor antagonist R817 (10(-6) M). In both VSMC preparations, the specific B1 agonist R211 (10(-9) to 10(-7) M) rapidly induced a nonsignificant increase of [Ca]c but a significant (p < 0.05) sustained increase of [Ca]n that was prevented but not reversed by the B1 selective antagonist R126 (10(-6) M). The sustained increase of [Ca]c and [Ca]n induced by BK and B1 receptor agonist was blocked by extracellular application of EGTA. These results strongly suggest that B1 and probably B2 receptors are functional in human and rabbit aortic VSMCs. BK-induced transient increase of [Ca]i is mainly due to the stimulation of T- and L-type Ica as well as to Ca2+ release from caffeine- and ryanodine-sensitive Ca2+ pools. The sustained component induced by the hormone or the B1 agonist is mainly nuclear and is due to the stimulation of Ca2+ influx through the R-type Ca2+ channels that are present at the sarcolemma and the nuclear membranes.
在人和兔主动脉血管平滑肌细胞(VSMCs)中研究了缓激肽(BK)刺激Ca2+内流的机制以及介导此效应的受体亚型。运用全细胞电压钳技术,BK(10(-6)M)可使兔主动脉VSMCs中的T型和L型Ca2+电流(ICa)显著(p < 0.05)增加。采用fura-2测量细胞内总Ca2+([Ca]i)的技术,BK(10(-6) M)可诱导[Ca]i先出现短暂升高,随后出现持续升高。用肌浆网(SR)Ca2+释放剂咖啡因(1 - 5 mM)预处理兔VSMCs,可显著降低BK诱导的[Ca]i短暂升高,但不影响该激素诱导的持续升高部分。该持续阶段可被细胞外应用Ca2+螯合剂EGTA阻断。运用fluo-3共聚焦显微镜测量Ca2+技术来定位胞质([Ca]c)和核内([Ca]n)游离Ca2+分布,兔和人主动脉VSMCs细胞质中Ca2+的静息持续浓度低于细胞核中的浓度。BK(10(-7) M)可诱导[Ca]c出现不显著的持续升高,但可诱导[Ca]n出现显著(p < 0.05)的持续升高,特异性B1受体拮抗剂R126(10(-6) M)以及B2受体拮抗剂R817(10(-6) M)可使其逆转但不能阻止。在两种VSMC制剂中,特异性B1激动剂R211(10(-9)至10(-7) M)可迅速诱导[Ca]c出现不显著的升高,但可诱导[Ca]n出现显著(p < 0.05)的持续升高,B1选择性拮抗剂R126(10(-6) M)可阻止但不能逆转这种升高。BK和B1受体激动剂诱导的[Ca]c和[Ca]n持续升高可被细胞外应用EGTA阻断。这些结果强烈提示B1受体以及可能的B2受体在人和兔主动脉VSMCs中发挥功能。BK诱导的[Ca]i短暂升高主要是由于T型和L型Ica的刺激以及咖啡因和ryanodine敏感Ca2+池释放Ca2+。该激素或B1激动剂诱导的持续升高部分主要在细胞核内,是由于通过存在于肌膜和核膜上 的R型Ca2+通道刺激Ca2+内流所致。
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