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蛋白激酶B/Akt2对胃酸分泌的调节

Regulation of gastric acid secretion by PKB/Akt2.

作者信息

Rotte Anand, Pasham Venkanna, Bhandaru Madhuri, Eichenmüller Melanie, Yang Wenting, Qadri Syed M, Kempe Daniela S, Puchchakayala Goverdhan, Pearce David, Birnbaum Morris J, Lang Florian

机构信息

Department of Physiology, University of Tübingen, D-72076 Tübingen, Germany.

出版信息

Cell Physiol Biochem. 2010;25(6):695-704. doi: 10.1159/000315089. Epub 2010 May 18.

Abstract

Pharmacological inhibition of phosphoinositol 3 kinase (PI3K) and partial deficiency of phosphoinositide dependent kinase PDK1 have previously been shown to enhance basal gastric acid secretion. PI3K/PDK1 dependent signaling involves activation of protein kinase B/Akt, which may thus be similarly involved in the regulation of gastric acid secretion. To test that hypothesis, gastric acid secretion was determined in isolated glands from gene targeted mice lacking functional Akt2 (akt2(-/-)) or from their wild type littermates (akt2(+/+)). According to BCECF-fluorescence cytosolic pH in isolated gastric glands was similar in akt2(-/-) and akt2(+/+) mice. Na(+)-independent pH recovery (DeltapH/min) following an ammonium pulse, a measure of H(+)/K(+) ATPase activity, was, however, significantly faster in akt2(-/-) than in akt2(+/+) mice. In both genotypes, DeltapH/min was virtually abolished by H(+)/K(+) ATPase inhibitor omeprazole (100 muM). Increase of extracellular K(+) concentrations to 35 mM (replacing Na(+)) increased DeltapH/min to a significantly larger extent in akt2(+/+) than in akt2(-/-) mice and dissipated the differences between the genotypes. Similarly, treatment with 5 muM forskolin enhanced DeltapH/min significantly only in akt2(+/+) mice and abolished the differences between the genotypes. Conversely, protein kinase A inhibitor H89 (50 nM) decreased DeltapH/min to similarly low values in both genotypes. In conclusion, Akt2 suppresses gastric acid secretion and contributes to or even accounts for the inhibition of gastric acid secretion by PI3K.

摘要

先前的研究表明,磷酸肌醇3激酶(PI3K)的药理学抑制和磷酸肌醇依赖性激酶PDK1的部分缺陷会增强基础胃酸分泌。PI3K/PDK1依赖性信号传导涉及蛋白激酶B/Akt的激活,因此其可能同样参与胃酸分泌的调节。为了验证这一假设,我们测定了基因靶向缺失功能性Akt2(akt2(-/-))的小鼠或其野生型同窝小鼠(akt2(+/+))分离腺体中的胃酸分泌。结果显示,akt2(-/-)和akt2(+/+)小鼠分离胃腺体中基于BCECF荧光的胞质pH相似。然而,铵脉冲后不依赖钠的pH恢复(ΔpH/分钟),即H(+)/K(+) ATP酶活性的一种测量方法,在akt2(-/-)小鼠中显著快于akt2(+/+)小鼠。在两种基因型中,H(+)/K(+) ATP酶抑制剂奥美拉唑(100 μM)几乎完全消除了ΔpH/分钟。将细胞外钾离子浓度增加到35 mM(替代钠离子)时,akt2(+/+)小鼠中ΔpH/分钟的增加幅度明显大于akt2(-/-)小鼠,并消除了基因型之间的差异。同样,用5 μM福司可林处理仅在akt2(+/+)小鼠中显著增强了ΔpH/分钟,并消除了基因型之间的差异。相反,蛋白激酶A抑制剂H89(50 nM)在两种基因型中将ΔpH/分钟降低到相似的低值。总之,Akt2抑制胃酸分泌,并对PI3K抑制胃酸分泌起到作用甚至起主要作用。

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