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铜绿假单胞菌脂氧合酶 Ala420Gly 突变体的晶体结构解释了其提高的氧亲和力和改变的反应特异性。

The crystal structure of Pseudomonas aeruginosa lipoxygenase Ala420Gly mutant explains the improved oxygen affinity and the altered reaction specificity.

机构信息

Institute of Medical Physics and Biophysics (CC2), Group Protein X-ray Crystallography and Signal Transduction, Charité - University Medicine Berlin, Charitéplatz 1, 10117 Berlin, Germany.

Institute for Biochemistry (CC2), Charité - University Medicine Berlin, Charitéplatz 1, 10117 Berlin, Germany.

出版信息

Biochim Biophys Acta Mol Cell Biol Lipids. 2017 May;1862(5):463-473. doi: 10.1016/j.bbalip.2017.01.003. Epub 2017 Jan 14.

DOI:10.1016/j.bbalip.2017.01.003
PMID:28093240
Abstract

Secreted LOX from Pseudomonas aeruginosa (PA-LOX) has previously been identified as arachidonic acid 15S-lipoxygenating enzyme. Here we report that the substitution of Ala420Gly in PA-LOX leads to an enzyme variant with pronounced dual specificity favoring arachidonic acid 11R-oxygenation. When compared with other LOX-isoforms the molecular oxygen affinity of wild-type PA-LOX is 1-2 orders of magnitude lower (Km O of 0.4mM) but Ala420Gly exchange improved the molecular oxygen affinity (Km O of 0.2mM). Experiments with stereo-specifically deuterated linoleic acid indicated that the formation of both 13S- and 9R-HpODE involves abstraction of the proS-hydrogen from C11 of the fatty acid backbone. To explore the structural basis for the observed functional changes (altered specificity, improved molecular oxygen affinity) we solved the crystal structure of the Ala420Gly mutant of PA-LOX at 1.8Å resolution and compared it with the wild-type enzyme. Modeling of fatty acid alignment at the catalytic center suggested that in the wild-type enzyme dioxygen is directed to C15 of arachidonic acid by a protein tunnel, which interconnects the catalytic center with the protein surface. Ala420Gly exchange redirects intra-enzyme O diffusion by bifurcating this tunnel so that C11 of arachidonic acid also becomes accessible for O insertion.

摘要

铜绿假单胞菌分泌的脂氧合酶(PA-LOX)先前被鉴定为花生四烯酸 15S-脂氧合酶。在这里,我们报告 PA-LOX 中的 Ala420Gly 取代导致酶变体具有明显的双重特异性,有利于花生四烯酸 11R-氧化。与其他 LOX 同工酶相比,野生型 PA-LOX 的分子氧亲和力低 1-2 个数量级(Km O 为 0.4mM),但 Ala420Gly 交换提高了分子氧亲和力(Km O 为 0.2mM)。用立体特异性氘化亚油酸进行的实验表明,13S-和 9R-HpODE 的形成都涉及从脂肪酸主链的 C11 上夺取 proS-氢。为了探索观察到的功能变化(改变的特异性、提高的分子氧亲和力)的结构基础,我们以 1.8Å 的分辨率解决了 Ala420Gly 突变型 PA-LOX 的晶体结构,并将其与野生型酶进行了比较。在催化中心对脂肪酸排列的建模表明,在野生型酶中,双原子氧被一条蛋白隧道引导至花生四烯酸的 C15,该隧道将催化中心与蛋白表面相互连接。Ala420Gly 交换通过分叉这条隧道来重新引导酶内 O 扩散,从而使花生四烯酸的 C11 也可用于 O 插入。

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