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金雀异黄素对囊性纤维化跨膜传导调节因子第二个核苷酸结合结构域的ATP酶、GTP酶和腺苷酸激酶活性的抑制作用。

Inhibition of ATPase, GTPase and adenylate kinase activities of the second nucleotide-binding fold of the cystic fibrosis transmembrane conductance regulator by genistein.

作者信息

Randak C, Auerswald E A, Assfalg-Machleidt I, Reenstra W W, Machleidt W

机构信息

Kinderklinik im Dr. von Haunerschen Kinderspital, Ludwig-Maximilians-Universität München, Lindwurmstrasse 4, D-80337 München, Germany.

出版信息

Biochem J. 1999 May 15;340 ( Pt 1)(Pt 1):227-35.

Abstract

In the presence of ATP, genistein, like the ATP analogue adenosine 5'-[beta,gamma-imido]triphosphate (pp[NH]pA), increases cystic fibrosis transmembrane conductance regulator (CFTR) chloride currents by prolonging open times. As pp[NH]pA is thought to increase CFTR currents by interfering with ATP hydrolysis at the second nucleotide-binding fold (NBF-2), the present study was undertaken to investigate the effects of genistein on a fusion protein comprising maltose-binding protein (MBP) and NBF-2 (MBP-NBF-2). MBP-NBF-2 exhibited ATPase, GTPase and adenylate kinase activities that were inhibited by genistein in a partial non-competitive manner with respect to ATP or GTP. Ki values for competitive and uncompetitive inhibition were respectively 20 microM and 63 microM for ATPase, 15 microM and 54 microM for GTPase, and 46 microM and 142 microM for adenylate kinase. For ATPase activity, genistein reduced Vmax by 29% and Vmax/Km by 77%. Additional evidence for complex-formation between genistein and MBP-NBF-2 was obtained by the detection of genistein-dependent alterations in the CD spectrum of MBP-NBF-2 that were consistent with the formation of a higher-ordered state. Addition of MBP-NBF-2 increased the fluorescence intensity of genistein, consistent with a change to a less polar environment. pp[NH]pA partially eliminated this enhanced fluorescence of genistein. These observations provide the first direct biochemical evidence that genistein interacts with CFTR, thus inhibiting NBF-2 activity, and suggest a similar mechanism for genistein-dependent stimulation of CFTR chloride currents.

摘要

在有ATP存在的情况下,染料木黄酮与ATP类似物腺苷5'-[β,γ-亚氨基]三磷酸(pp[NH]pA)一样,通过延长开放时间来增加囊性纤维化跨膜传导调节因子(CFTR)的氯离子电流。由于认为pp[NH]pA通过干扰第二个核苷酸结合结构域(NBF-2)处的ATP水解来增加CFTR电流,因此进行了本研究以调查染料木黄酮对包含麦芽糖结合蛋白(MBP)和NBF-2(MBP-NBF-2)的融合蛋白的影响。MBP-NBF-2表现出ATP酶、GTP酶和腺苷酸激酶活性,这些活性被染料木黄酮以对ATP或GTP部分非竞争性的方式抑制。ATP酶竞争性和非竞争性抑制的Ki值分别为20μM和63μM,GTP酶分别为15μM和54μM,腺苷酸激酶分别为46μM和142μM。对于ATP酶活性,染料木黄酮使Vmax降低29%,Vmax/Km降低77%。通过检测MBP-NBF-2的圆二色光谱中与更高有序状态形成一致的染料木黄酮依赖性变化,获得了染料木黄酮与MBP-NBF-2之间形成复合物的额外证据。添加MBP-NBF-2增加了染料木黄酮的荧光强度,这与向极性较小的环境转变一致。pp[NH]pA部分消除了染料木黄酮这种增强的荧光。这些观察结果提供了首个直接的生化证据,表明染料木黄酮与CFTR相互作用,从而抑制NBF-2活性,并提示了染料木黄酮依赖性刺激CFTR氯离子电流的类似机制。

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