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Inhibition of small-conductance Cl− channels by the interleukin-1β-stimulated production of superoxide in rabbit gastric parietal cells

机译:白介素-1β刺激兔胃壁细胞超氧化物生成对小传导性Cl-通道的抑制

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摘要

We have shown previously that the G protein-coupled production of superoxide anion (O2) leads to closure of small-conductance Cl channels (0.3–0.4 pS) in the basolateral membrane of rabbit parietal cells. In the present study, effects of interleukin-1β (IL-1β) on the Cl channel were investigated. In the whole-cell patch-clamp recording, IL-1β (0.3–10 ng ml−1) inhibited the whole-cell Cl current recorded from a parietal cell within isolated rabbit gastric glands. Variance noise analysis of the whole-cell Cl current showed that the single channel conductance of the Cl channel that is sensitive to IL-1β is 0.37 pS. The IL-1β (1 ng ml−1)-induced decrease of the Cl current was abolished by anti-IL-1β antibody (2 μg ml−1), recombinant IL-1 receptor antagonist (500 ng ml−1), GDPβS (500 μM) and superoxide dismutase (100 units ml−1), a scavenger of O2. Northern blot analysis showed that the mRNA of the IL-1 receptor was selectively expressed in rabbit gastric parietal cells. In the dihydrofluorescein diacetate-loaded single parietal cells in gastric glands, IL-1β (0.3–10 ng ml−1) stimulated the production of oxygen radicals. Y-27632 (1–10 μM), a specific Rho-kinase inhibitor, and fluvastatin (10 μM), an indirect inhibitor for Rho proteins, significantly inhibited the IL-1β-induced effects on the channel activity and production of oxygen radicals. IL-1β (0.3–10 ng ml−1) activated Rho in the parietal cells. These results indicate that IL-1β binds to the IL-1 receptor of gastric parietal cells and inhibits the small-conductance Cl channel via the G protein-mediated Rho/Rho-kinase-dependent production of O2.
机译:先前我们已经表明,G蛋白偶联的超氧阴离子(O2 -)的产生导致小导电Cl -通道(0.3–0.4 pS)的关闭。兔壁细胞的基底外侧膜。在本研究中,研究了白介素-1β(IL-1β)对Cl -通道的影响。在全细胞膜片钳记录中,IL-1β(0.3–10 ng ml -1 )抑制了从壁细胞中记录的全细胞Cl -电流离体的兔胃腺。对全细胞Cl -电流的方差噪声分析表明,对IL-1β敏感的Cl -通道的单通道电导为0.37 pS。 IL-1β(1 ng ml -1 )诱导的Cl -电流降低被抗IL-1β抗体(2μgml - 1 ),重组IL-1受体拮抗剂(500 ng ml -1 ),GDPβS(500μM)和超氧化物歧化酶(100单位ml -1 ) ,是O2 -的清除剂。 Northern印迹分析表明,IL-1受体的mRNA在家兔胃壁细胞中选择性表达。在胃腺中的二乙酸二氢荧光素单壁细胞中,IL-1β(0.3–10 ng ml −1 )刺激了氧自由基的产生。特定的Rho激酶抑制剂Y-27632(1–10μM)和Rho蛋白的间接抑制剂氟伐他汀(10μM)显着抑制IL-1β诱导的对通道活性和氧自由基产生的影响。 IL-1β(0.3–10 ng ml -1 )激活顶细胞中的Rho。这些结果表明,IL-1β结合胃壁细胞的IL-1受体,并通过G蛋白介导的Rho / Rho激酶依赖性O2的产生抑制小电导Cl -通道。 -

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