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花生四烯酸对豚鼠输精管单个平滑肌细胞钙通道电流的调制作用

Modulation of calcium channel currents by arachidonic acid in single smooth muscle cells from vas deferens of the guinea-pig.

作者信息

Nagano N, Imaizumi Y, Watanabe M

机构信息

Department of Chemical Pharmacology, Faculty of Pharmacentical Science, Nagoya City University, Japan.

出版信息

Br J Pharmacol. 1995 Sep;116(2):1887-93. doi: 10.1111/j.1476-5381.1995.tb16678.x.

Abstract
  1. Effects of arachidonic acid (AA) on voltage-dependent Ca channel currents were investigated by whole-cell-clamp methods in single smooth muscle cells freshly isolated from vas deferens of the guinea-pig. 2. Ca channel current was decreased by application of 1-30 microM AA in a concentration-dependent manner. When Ca2+ or Ba2+ was the charge carrier, Ca channel current (ICa or IBa) was reduced by AA to a similar extent (IC50 = 10 and 6 microM, respectively). Addition of 15 mM BAPTA to the pipette solution did not affect the reduction of IBa by 10 microM AA. 3. The effect of AA on IBa was not prevented by internal application of 1 mM nordihydroguaiaretic acid (NDGA) and 1 mM indomethacin (Indo). When the pipette solution contained 0.1 mM guanosine-5'-triphosphate (GTP), IBa was decreased slightly but significantly by application of 30 microM prostaglandin F2 alpha (PGF2 alpha) but not by PGE2. This effect of PGF2 alpha was irreversible or not observed when the pipette solution contained 0.3 mM guanosine-5'-(3-thiotriphosphate) (GTP gamma S) or both GTP or guanosine-5'-O-(2-thiodiphosphate) (GDP beta S), respectively. 4. External application of 100 units ml-1 superoxide dismutase slightly but significantly attenuated the inhibition of IBa by 1-30 microM AA. Intracellular application of 1 mM GDP beta S or 0.3 mM GTP gamma S did not significantly change the effect of AA. Intracellular application of 0.1 mM 1-(5-isoquinolinesulphonyl)-2-methylepiperazine (H-7) also did not change the effect of AA. 5. These results indicate that the decrease in Ca channel currents in vas deferens smooth muscle cells is mainly due to AA itself, as opposed to its metabolites. The effect of AA may be due to AA itself, as opposed to its metabolites. The effect of AA may be due to its direct action on Ca channels or membrane phospholipids, but may not be mediated by activation of GTP binding proteins or protein kinase C. The inhibition of Ca channel current by AA may be partly induced by superoxide radicals derived from AA oxidation. PGF2A also reduces Ca channel currents but probably by a separate mechanism via activation of a GTP binding protein.
摘要
  1. 采用全细胞钳制方法,在从豚鼠输精管新鲜分离的单个平滑肌细胞中研究了花生四烯酸(AA)对电压依赖性钙通道电流的影响。2. 应用1 - 30微摩尔/升的AA可使钙通道电流以浓度依赖性方式降低。当Ca2+或Ba2+作为载流子时,AA使钙通道电流(ICa或IBa)降低的程度相似(IC50分别为10和6微摩尔/升)。向微电极溶液中添加15毫摩尔/升的BAPTA并不影响10微摩尔/升AA对IBa的降低作用。3. 细胞内应用1毫摩尔/升去甲二氢愈创木酸(NDGA)和1毫摩尔/升吲哚美辛(Indo)并不能阻止AA对IBa的作用。当微电极溶液中含有0.1毫摩尔/升鸟苷 - 5'-三磷酸(GTP)时,应用30微摩尔/升前列腺素F2α(PGF2α)可使IBa轻微但显著降低,而PGE2则无此作用。当微电极溶液分别含有0.3毫摩尔/升鸟苷 - 5'-(3 - 硫代三磷酸)(GTPγS)或同时含有GTP或鸟苷 - 5'-O-(2 - 硫代二磷酸)(GDPβS)时,PGF2α的这种作用不可逆或未观察到。4. 细胞外应用100单位/毫升超氧化物歧化酶可轻微但显著减弱1 - 30微摩尔/升AA对IBa的抑制作用。细胞内应用1毫摩尔/升GDPβS或0.3毫摩尔/升GTPγS并没有显著改变AA的作用。细胞内应用0.1毫摩尔/升1 - (5 - 异喹啉磺酰基)-2 - 甲基哌嗪(H - 7)也没有改变AA的作用。5. 这些结果表明,输精管平滑肌细胞中钙通道电流的降低主要是由于AA本身,而非其代谢产物。AA的作用可能归因于其本身,而非其代谢产物。AA的作用可能是由于其对钙通道或膜磷脂的直接作用,但可能不是由GTP结合蛋白或蛋白激酶C的激活介导的。AA对钙通道电流的抑制作用可能部分是由AA氧化产生的超氧自由基诱导的。PGF2A也可降低钙通道电流,但可能是通过激活GTP结合蛋白的另一种机制。

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