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焦磷酸产生的质子电化学梯度对红甜菜液泡膜H(+)-ATP酶的逆转作用。

Reversal of the red beet tonoplast H(+)-ATPase by a pyrophosphate-generated proton electrochemical gradient.

作者信息

Schmidt A L, Briskin D P

机构信息

Department of Agronomy, University of Illinois, Urbana 61801.

出版信息

Arch Biochem Biophys. 1993 Nov 1;306(2):407-14. doi: 10.1006/abbi.1993.1530.

Abstract

The reversal of the tonoplast H(+)-ATPase to mediate ATP synthesis was investigated in tonoplast vesicles isolated from red beet (Beta vulgaris L.) storage tissue. Our approach involved use of the H(+)-PP(i)ase to establish a proton electrochemical gradient (delta muH+) across the tonoplast vesicle membrane to drive the H(+)-ATPase in reverse. However, an initial problem with this approach was the presence of an adenylate kinase activity in the tonoplast fraction that interfered with measurement of ATP synthesis as a coupling between the H(+)-ATPase and H(+)-PP(i)ase. Inclusion of the adenylate kinase inhibitor p1p5-di(adenosine)pentaphosphate (Ap5A) in assays at 50 microM led to a complete inhibition of this activity and allowed measurement of ATP synthesis coupled to PPi hydrolysis. When measured in the presence of Ap5A, PPi-dependent ATP synthesis was blocked by Triton X-100 and inhibited by gramicidin D, imidodiphosphate, nitrate, and bafilomycin A. These results are consistent with PPi-dependent ATP synthesis occurring as a coupled process involving a delta muH+ established across the membrane. Furthermore, the observation that ATP synthesis is inhibited by inhibitors of the tonoplast H(+)-ATPase (nitrate and bafilomycin A) would suggest that this enzyme is involved in the synthetic reaction and can operate in reverse to synthesize ATP from ADP and Pi. A thermodynamic analysis of coupling between the H(+)-PP(i)ase and H(+)-ATPase suggests that PPi-driven ATP synthesis could only occur under these reaction conditions if the H+/substrate stoichiometries for the H(+)-PP(i)ase and H(+)-ATPase were 1 and 2, respectively. These values are consistent with transport stoichiometries previously determined for these enzymes in red beet tonoplast vesicles using kinetic methods.

摘要

在从红甜菜(Beta vulgaris L.)贮藏组织分离的液泡膜囊泡中,研究了液泡膜H(+)-ATP酶介导ATP合成的逆转情况。我们的方法是利用H(+)-PP(i)酶在液泡膜囊泡膜上建立质子电化学梯度(δμH+),以反向驱动H(+)-ATP酶。然而,这种方法最初的一个问题是液泡膜部分存在腺苷酸激酶活性,它干扰了作为H(+)-ATP酶和H(+)-PP(i)酶偶联反应的ATP合成的测量。在测定中加入50微摩尔的腺苷酸激酶抑制剂p1p5-二(腺苷)五磷酸(Ap5A),可完全抑制该活性,并能测量与PPi水解偶联的ATP合成。当在Ap5A存在下进行测量时,PPi依赖的ATP合成被 Triton X-100阻断,并被短杆菌肽D、亚氨二磷酸、硝酸盐和巴弗洛霉素A抑制。这些结果与PPi依赖的ATP合成作为一个涉及跨膜建立的δμH+的偶联过程发生是一致的。此外,液泡膜H(+)-ATP酶抑制剂(硝酸盐和巴弗洛霉素A)抑制ATP合成的观察结果表明,该酶参与了合成反应,并且可以反向运作以从ADP和Pi合成ATP。对H(+)-PP(i)酶和H(+)-ATP酶之间偶联的热力学分析表明,只有当H(+)-PP(i)酶和H(+)-ATP酶的H+/底物化学计量比分别为1和2时,PPi驱动的ATP合成才可能在这些反应条件下发生。这些值与先前使用动力学方法在红甜菜液泡膜囊泡中测定的这些酶的转运化学计量比一致。

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