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Activation of small conductance Ca(2+)-dependent K+ channels by purinergic agonists in smooth muscle cells of the mouse ileum.

机译:嘌呤激动剂在小鼠回肠平滑肌细胞中的小电导Ca(2+)依赖性K +通道的激活。

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摘要

1. Whole-cell and single-channel K+ currents were recorded at room temperature (22-24 degrees C), from smooth muscle cells enzymatically dispersed from the mouse ileum, using variations of the patch-clamp technique. 2. Net outward K+ currents recorded through amphotericin-B-perforated patches in response to step depolarizations positive to -50 mV from a holding potential of -80 mV were decreased by up to 70% by external apamin (0.5 microM). Apamin-sensitive whole-cell currents were also recorded from cells perfused internally with 150 nM Ca2+ but not from cells perfused internally with 85 nM Ca2+. 3. Three types of non-inactivating Ca(2+)-sensitive K+ channels were identified in cell-attached and excised patches under an asymmetrical K+ gradient: (i) large conductance (BKCa; approximately 200 pS) channels blocked by 2 mM external TEA; (ii) intermediate conductance (IKCa; approximately 39 pS) channels blocked by 2 mM external TEA and inhibited by external apamin (0.5 microM); and (iii) small conductance (SKCa; approximately 10 pS) channels that were not blocked by 5 mM external TEA but were sensitive to extracellular apamin (0.5 microM). 4. The TEA-resistant SKCa channels were activated by an increase in [Ca2+]i with an EC50 of 1.5 microM and a Hill coefficient of 1.3. 5. P2 purinoceptor agonists 2-methylthioATP (2-MeSATP), 2-chloroATP and ATP (10-50 microM) increased an apamin-sensitive whole-cell outward K+ current. Extrapatch application of 2-MeSATP (20-100 microM) stimulated the apamin-sensitive IKCa and SKCa channels and activated an apamin-sensitive steady outward current at 0 mV. 6. Smooth muscle cells from the mouse ileum possess two apamin-sensitive K+ channels (IKCa and SKCa); of these, the IKCa channels are TEA sensitive while the SKCa channels are TEA resistant. These channels, along with an apamin-sensitive but TEA-resistant steady outward current, may mediate membrane hyperpolarization elicited by purinergic agonists.
机译:1.在室温(22-24摄氏度)下,使用膜片钳技术的变化,从小鼠回肠中酶促分散的平滑肌细胞中记录全细胞和单通道K +电流。 2.通过两性霉素B穿孔的贴片记录的净向外K +电流,响应于从-80 mV的保持电势到-50 mV的逐步去极化,通过外部木瓜蛋白酶(0.5 microM)降低了70%。还记录了从内部用150 nM Ca2 +灌注的细胞对糊精敏感的全细胞电流,但没有从内部用85 nM Ca2 +灌注的细胞记录。 3.在非对称K +梯度下,在细胞附着和切除的斑块中鉴定出三种非灭活的Ca(2+)敏感K +通道:(i)大电导(BKCa;约200 pS)通道被2 mM外部阻滞茶; (ii)中间电导(IKCa;约39 pS)通道被2 mM外部TEA阻断并被外部阿帕明(0.5 microM)抑制; (iii)小电导(SKCa;大约10 pS)通道,不受5 mM外部TEA阻滞,但对细胞外Apapamin(0.5 microM)敏感。 4. TEA耐药SKCa通道通过[Ca2 +] i的增加而激活,EC50为1.5 microM,希尔系数为1.3。 5. P2嘌呤受体激动剂2-methylthioATP(2-MeSATP),2-chloroATP和ATP(10-50 microM)增加了对罂粟碱敏感的全细胞向外K +电流。 2-MeSATP(20-100 microM)的超补剂施用刺激了对糊精敏感的IKCa和SKCa通道,并在0 mV激活了对糊精敏感的稳定向外电流。 6.来自小鼠回肠的平滑肌细胞具有两个对apapamin敏感的K +通道(IKCa和SKCa);其中,IKCa通道对TEA敏感,而SKCa通道对TEA敏感。这些通道,以及对apapa敏感但对TEA耐受的稳定的向外电流,可能介导嘌呤能激动剂引起的膜超极化。

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    Vogalis, F; Goyal, R K;

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  • 年度 1997
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