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海分枝杆菌 CYP105Q4 细胞色素 P450 酶的结构测定与特性研究。

Structural determination and characterisation of the CYP105Q4 cytochrome P450 enzyme from Mycobacterium marinum.

机构信息

Department of Chemistry, University of Adelaide, SA, 5005, Australia.

School of Biological Sciences, University of Adelaide, SA, 5005, Australia.

出版信息

Arch Biochem Biophys. 2024 Apr;754:109950. doi: 10.1016/j.abb.2024.109950. Epub 2024 Feb 29.

DOI:10.1016/j.abb.2024.109950
PMID:38430969
Abstract

The cytochrome P450 family of heme metalloenzymes (CYPs) catalyse important biological monooxygenation reactions. Mycobacterium marinum contains a gene encoding a CYP105Q4 enzyme of unknown function. Other members of the CYP105 CYP family have key roles in bacterial metabolism including the synthesis of secondary metabolites. We produced and purified the cytochrome P450 enzyme CYP105Q4 to enable its characterization. Several nitrogen-donor atom-containing ligands were found to bind to CYP105Q4 generating type II changes in the UV-vis absorbance spectrum. Based on the UV-vis absorbance spectra none of the potential substrate ligands we tested with CYP105Q4 were able to displace the sixth distal aqua ligand from the heme, though there was evidence for binding of oleic acid and amphotericin B. The crystal structure of CYP105Q4 in the substrate-free form was determined in an open conformation. A computational structural similarity search (Dali) was used to find the most closely related characterized relatives within the CYP105 family. The structure of CYP105Q4 enzyme was compared to the GfsF CYP enzyme from Streptomyces graminofaciens which is involved in the biosynthesis of a macrolide polyketide. This structural comparison to GfsF revealed conformational changes in the helices and loops near the entrance to the substrate access channel. A disordered B/C loop region, usually involved in substrate recognition, was also observed.

摘要

细胞色素 P450 家族的血红素金属酶 (CYPs) 催化重要的生物单加氧反应。海洋分枝杆菌含有编码一种未知功能的 CYP105Q4 酶的基因。CYP105 CYP 家族的其他成员在细菌代谢中起着关键作用,包括次生代谢物的合成。我们生产并纯化了细胞色素 P450 酶 CYP105Q4,以对其进行表征。发现几种含氮供原子的配体与 CYP105Q4 结合,在紫外可见吸收光谱中产生 II 型变化。根据紫外可见吸收光谱,我们用 CYP105Q4 测试的潜在底物配体都不能从血红素中置换出第六个远端水合配体,尽管有油酸和两性霉素 B 结合的证据。在无底物形式下,CYP105Q4 的晶体结构被确定为开放构象。进行了计算结构相似性搜索 (Dali),以找到 CYP105 家族中最密切相关的特征亲属。将 CYP105Q4 酶的结构与参与大环内酯聚酮生物合成的来自链霉菌属的 GfsF CYP 酶进行比较。与 GfsF 的这种结构比较揭示了底物进入通道入口附近的螺旋和环的构象变化。还观察到通常涉及底物识别的无序 BC 环区。

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