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二苯乙烯基雌二醇对燕麦根质膜部分三磷酸腺苷酶活性的抑制作用。

Inhibition of adenosine triphosphatase activity of the plasma membrane fraction of oat roots by diethylstilbestrol.

机构信息

Department of Botany and Plant Pathology, Purdue University, West Lafayette, Indiana 47907.

出版信息

Plant Physiol. 1979 Jan;63(1):48-52. doi: 10.1104/pp.63.1.48.

Abstract

Diethylstibestrol (DES) inhibited noncompetitively the ATPase in the plasma membrane fraction from Avena sativa L. cv. Goodfield roots when assayed in the presence of MgSO(4) or MgSO(4) plus KCl. In the presence of MgSO(4), 7.1x10(-5) molar DES inhibited the enzyme 50%; whereas in the presence of MgSO(4) and KCl, 1.3x10(-4) molar DES was required for the same inhibition. Dixon plots indicated that in the presence of MgSO(4), one molecule of DES bound to one molecule of ATPase; however, in the presence of MgSO(4) and KCl, two or more molecules bound to one ATPase molecule. These results suggested that KCl causes a conformational change in the enzyme which exposes additional binding sites for DES, but that these sites are not as inhibitory as the first binding site.In addition to KCl, other factors also affected the DES inhibition of the ATPase. Plasma membrane vesicles warmed to 38 C were inhibited more than vesicles kept on ice prior to assay. DES inhibited the Triton X-100-treated ATPase less than the ATPase which was not detergent-treated. Finally, studies with DES analogs showed that the hydroxyl groups of DES were essential for inhibition and that steric configurations of the molecule were important.DES inhibition of the ATPase suggests that DES inhibits K(+) absorption in oat roots by inhibiting the ATPase. Inhibition of K(+) absorption was greater than inhibition of the ATPase, and thus DES may also inhibit other aspects of metabolism that are involved with ion absorption.

摘要

己烯雌酚(DES)在存在 MgSO4 或 MgSO4 和 KCl 时,非竞争性地抑制了来自 Avena sativa L. cv. Goodfield 根质膜部分的 ATP 酶。在存在 MgSO4 的情况下,7.1x10(-5)摩尔 DES 抑制了 50%的酶;而在存在 MgSO4 和 KCl 的情况下,需要 1.3x10(-4)摩尔 DES 才能达到相同的抑制效果。Dixon 图表明,在存在 MgSO4 的情况下,一个 DES 分子与一个 ATP 酶分子结合;然而,在存在 MgSO4 和 KCl 的情况下,两个或更多的分子与一个 ATP 酶分子结合。这些结果表明,KCl 导致酶的构象发生变化,暴露出更多的 DES 结合位点,但这些位点不如第一个结合位点具有抑制作用。除了 KCl 之外,其他因素也影响了 DES 对 ATP 酶的抑制作用。与在测定前保持在冰上的囊泡相比,加热至 38°C 的质膜囊泡受到的抑制作用更大。DES 对 Triton X-100 处理的 ATP 酶的抑制作用小于未用去污剂处理的 ATP 酶。最后,用 DES 类似物进行的研究表明,DES 抑制了 K(+)吸收,这是因为它抑制了 ATP 酶。K(+)吸收的抑制作用大于 ATP 酶的抑制作用,因此 DES 可能还抑制了与离子吸收有关的代谢的其他方面。

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