控制咖啡因诱导猪冠状动脉舒张的机制。

Mechanisms controlling caffeine-induced relaxation of coronary artery of the pig.

作者信息

van der Bent V, Bény J L

机构信息

University of Geneva, Dept. of Zoology and Animal Biology, Switzerland.

出版信息

Br J Pharmacol. 1991 Aug;103(4):1877-82. doi: 10.1111/j.1476-5381.1991.tb12345.x.

DOI:10.1111/j.1476-5381.1991.tb12345.x

PMID:1912976

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1908191/

Abstract

We studied the effects of caffeine on coronary artery smooth muscle of the pig by measuring changes in isometric tension, cytosolic free Ca(2+) concentration ( [Ca2+]i) and transmembrane potential. 2. In the absence of tone, caffeine induced a concentration-dependent transient contraction of coronary artery strips, followed by sustained relaxation. Simultaneously with the relaxation, caffeine, 25 mM, hyperpolarized the smooth muscle cells by 7.7 +/- 0.9 mV. 3. Caffeine caused a concentration-dependent relaxation of strips precontracted with 10(-5)M acetylcholine (ACH). A supramaximal relaxing concentration of 25 mM caffeine produced an additional transient increase in [Ca2+]i on the Ca2+ plateau of ACh tonic contraction, which was followed by a decrease in [Ca2+]i to a level slightly below the basal concentration. This relaxation was accompanied by a hyperpolarization of 7.3 +/- 0.9 mV. 4. KCI 120 mM (high K+) contracted the strips with a concomitant depolarization of 38.6 +/- 1.6 mV and sustained increase in [Ca2+]i. Caffeine caused a concentration-dependent relaxation of high K+-induced contraction. Caffeine, 25 mM, decreased the Ca2+ plateau to a level that remained above the basal concentration of Ca2+ but did not change the membrane potential. 5. When strips were placed in a Ca(2+)-free medium with EGTA 2mM, and, in addition, ACh was applied successively three times, both intracellular and extracellular mobilizable Ca2+ pools were depleted. In these conditions, phorbol 12,13 dibutyrate (PDBu) 10(-7) M and prostaglandin F 2 alpha (PGF 2 alpha) 10(-5) M contracted the strips. Caffeine (25 mM) inhibited these contractions with no change in [Ca2+]i. 6. Forskolin, 3 x 10 -7M, inhibited ACh induced-contraction but did not affect those induced by PDBu. 7. In conclusion, these results show that caffeine has multiple cellular effects. During caffeine-induced relaxation, [Ca2" Ii, adenosine 3': 5'-cyclic monophosphate (cyclic AMP) content and membrane potential are modified. The findings suggest, however, that these effects are secondary, and that caffeine acts mainly by another unknown mechanism, possibly involving a direct inhibition of the contractile apparatus.

摘要

我们通过测量等长张力、胞质游离钙（Ca2+）浓度（[Ca2+]i）和跨膜电位的变化，研究了咖啡因对猪冠状动脉平滑肌的影响。2. 在无张力状态下，咖啡因引起冠状动脉条带浓度依赖性的短暂收缩，随后是持续性舒张。在舒张的同时，25 mM咖啡因使平滑肌细胞超极化7.7±0.9 mV。3. 咖啡因使预先用10-5M乙酰胆碱（ACH）预收缩的条带产生浓度依赖性舒张。25 mM咖啡因的最大舒张浓度在ACH张力性收缩的Ca2+平台上使[Ca2+]i额外短暂增加，随后[Ca2+]i降至略低于基础浓度的水平。这种舒张伴随着7.3±0.9 mV的超极化。4. 120 mM KCl（高钾）使条带收缩，同时去极化38.6±1.6 mV，并使[Ca2+]i持续增加。咖啡因使高钾诱导的收缩产生浓度依赖性舒张。25 mM咖啡因使Ca2+平台降至仍高于Ca2+基础浓度但不改变膜电位的水平。5. 当条带置于含2 mM EGTA的无钙培养基中，并且ACH连续施加三次时，细胞内和细胞外可动员的Ca2+池均被耗尽。在这些条件下，10-7M佛波醇12,13 -二丁酸酯（PDBu）和10-5M前列腺素F2α（PGF2α）使条带收缩。25 mM咖啡因抑制这些收缩，而[Ca2+]i无变化。6. 3×10-7M福斯高林抑制ACH诱导的收缩，但不影响PDBu诱导的收缩。7. 总之，这些结果表明咖啡因具有多种细胞效应。在咖啡因诱导的舒张过程中，[Ca2+]i、腺苷3':5'-环磷酸（环磷酸腺苷）含量和膜电位发生改变。然而，这些发现表明这些效应是次要的，并且咖啡因主要通过另一种未知机制起作用，可能涉及对收缩装置的直接抑制。