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泰国伯克霍尔德菌MSMB121中烷烃单加氧酶的同源建模与蛋白质工程:计算机模拟见解

Homology modeling and protein engineering of alkane monooxygenase in Burkholderia thailandensis MSMB121: in silico insights.

作者信息

Jain Chakresh Kumar, Gupta Money, Prasad Yamuna, Wadhwa Gulshan, Sharma Sanjeev Kumar

机构信息

Department of Biotechnology, Jaypee Institute of Information Technology, A-10, Sector-62, NOIDA, Uttar Pradesh, 201307, India,

出版信息

J Mol Model. 2014 Jul;20(7):2340. doi: 10.1007/s00894-014-2340-3. Epub 2014 Jul 3.

DOI:10.1007/s00894-014-2340-3
PMID:24990796
Abstract

The degradation of hydrocarbons plays an important role in the eco-balancing of petroleum products, pesticides and other toxic products in the environment. The degradation of hydrocarbons by microbes such as Geobacillus thermodenitrificans, Burkhulderia, Gordonia sp. and Acinetobacter sp. has been studied intensively in the literature. The present study focused on the in silico protein engineering of alkane monooxygenase (ladA)-a protein involved in the alkane degradation pathway. We demonstrated the improvement in substrate binding energy with engineered ladA in Burkholderia thailandensis MSMB121. We identified an ortholog of ladA monooxygenase found in B. thailandensis MSMB121, and showed it to be an enzyme involved in an alkane degradation pathway studied extensively in Geobacillus thermodenitrificans. Homology modeling of the three-dimensional structure of ladA was performed with a crystal structure (protein databank ID: 3B9N) as a template in MODELLER 9v11, and further validated using PROCHECK, VERIFY-3D and WHATIF tools. Specific amino acids were substituted in the region corresponding to amino acids 305-370 of ladA protein, resulting in an enhancement of binding energy in different alkane chain molecules as compared to wild protein structures in the docking experiments. The substrate binding energy with the protein was calculated using Vina (Implemented in VEGAZZ). Molecular dynamics simulations were performed to study the dynamics of different alkane chain molecules inside the binding pockets of wild and mutated ladA. Here, we hypothesize an improvement in binding energies and accessibility of substrates towards engineered ladA enzyme, which could be further facilitated for wet laboratory-based experiments for validation of the alkane degradation pathway in this organism.

摘要

碳氢化合物的降解在石油产品、农药及环境中其他有毒产品的生态平衡中发挥着重要作用。诸如嗜热脱氮地芽孢杆菌、伯克霍尔德菌、戈登氏菌属和不动杆菌属等微生物对碳氢化合物的降解已在文献中得到深入研究。本研究聚焦于烷烃单加氧酶(ladA)的计算机辅助蛋白质工程,ladA是一种参与烷烃降解途径的蛋白质。我们证明了泰国伯克霍尔德菌MSMB121中经工程改造的ladA的底物结合能有所提高。我们鉴定出泰国伯克霍尔德菌MSMB121中ladA单加氧酶的一个直系同源物,并表明它是一种在嗜热脱氮地芽孢杆菌中得到广泛研究的参与烷烃降解途径的酶。在MODELLER 9v11中,以晶体结构(蛋白质数据库ID:3B9N)为模板对ladA的三维结构进行同源建模,并使用PROCHECK、VERIFY-3D和WHATIF工具进行进一步验证。在与ladA蛋白第305 - 370位氨基酸对应的区域替换特定氨基酸,与对接实验中的野生型蛋白质结构相比,不同烷烃链分子的结合能有所增强。使用Vina(在VEGAZZ中实现)计算蛋白质与底物的结合能。进行分子动力学模拟以研究野生型和突变型ladA结合口袋内不同烷烃链分子的动力学。在此,我们推测工程改造后的ladA酶的结合能和底物可及性有所提高,并可进一步推动基于湿实验室的实验,以验证该生物体中的烷烃降解途径。

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