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将食油假单胞菌烷烃ω-羟化酶(一种整合膜二铁酶)与脂肪酸去饱和酶家族联系起来的证据。

Evidence linking the Pseudomonas oleovorans alkane omega-hydroxylase, an integral membrane diiron enzyme, and the fatty acid desaturase family.

作者信息

Shanklin John, Whittle Edward

机构信息

Department of Biology, Brookhaven National Laboratory, Building 463, 50 Bell Ave., Upton, NY 11973, USA.

出版信息

FEBS Lett. 2003 Jun 19;545(2-3):188-92. doi: 10.1016/s0014-5793(03)00529-5.

Abstract

Pseudomonas oleovorans alkane omega-hydroxylase (AlkB) is an integral membrane diiron enzyme that shares a requirement for iron and oxygen for activity in a manner similar to that of the non-heme integral membrane desaturases, epoxidases, acetylenases, conjugases, ketolases, decarbonylase and methyl oxidases. No overall sequence similarity is detected between AlkB and these desaturase-like enzymes by computer algorithms; however, they do contain a series of histidine residues in a similar relative positioning with respect to hydrophobic regions thought to be transmembrane domains. To test whether these conserved histidine residues are functionally equivalent to those of the desaturase-like enzymes we used scanning alanine mutagenesis to test if they are essential for activity of AlkB. These experiments show that alanine substitution of any of the eight conserved histidines results in complete inactivation, whereas replacement of three non-conserved histidines in close proximity to the conserved residues, results in only partial inactivation. These data provide the first experimental support for the hypotheses: (i) that the histidine motif in AlkB is equivalent to that in the desaturase-like enzymes and (ii) that the conserved histidine residues play a vital role such as coordinating the Fe ions comprising the diiron active site.

摘要

食油假单胞菌烷烃ω-羟化酶(AlkB)是一种整合膜双铁酶,其活性对铁和氧的需求方式与非血红素整合膜去饱和酶、环氧化酶、乙炔酶、共轭酶、酮醇酶、脱羰酶和甲基氧化酶类似。通过计算机算法未检测到AlkB与这些去饱和酶样酶之间存在整体序列相似性;然而,它们确实在相对于被认为是跨膜结构域的疏水区域的相似相对位置上含有一系列组氨酸残基。为了测试这些保守的组氨酸残基在功能上是否等同于去饱和酶样酶的残基,我们使用扫描丙氨酸诱变来测试它们对AlkB活性是否至关重要。这些实验表明,八个保守组氨酸中的任何一个被丙氨酸取代都会导致完全失活,而在保守残基附近的三个非保守组氨酸被取代只会导致部分失活。这些数据为以下假设提供了首个实验支持:(i)AlkB中的组氨酸基序与去饱和酶样酶中的组氨酸基序等同;(ii)保守的组氨酸残基发挥着至关重要的作用,例如配位构成双铁活性位点的铁离子。

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