一种新的抗菌药物靶点——单核增生李斯特菌choris酸合成酶的结构分析及潜在配体的分子对接。

IF 1.5 4区生物学 Q4 BIOCHEMISTRY & MOLECULAR BIOLOGY

Indian journal of biochemistry & biophysics Pub Date : 2015-02-01

Md Musharaf Hossain, Pradip Kumar Roy, A T M Jannatul Mosnaz, Shahriar Kabir Shakil, Md Mehedi Hasan, Shamsul H Prodhan

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引用次数: 0

摘要

李斯特菌病，特别是由单核细胞增生李斯特菌引起的李斯特菌病，是一种主要的食源性病原体，由于耐药菌株的广泛出现，控制李斯特菌病变得越来越困难。甘草酸合成酶(Chorismate synthase, CS)是一种仅存在于细菌、真菌、植物和一些顶复合体寄生虫中的莽草酸途径必需酶，是一种经过验证的潜在抗菌药物靶点。通过对单核增生L. L.单核增生L. L.单核增生L. L. L.单核增生L. L. L.单核增生L. L. L. L.单核增生L. L. L. L. L.单核增生L. L. LmCS的主要结构特征的阐明，进行抗菌开发，鉴定和优选潜在的靶向LmCS先导化合物。使用Autodock工具进行基于结构的虚拟筛选和对接研究，从几个配体库中检索对LmCS模型具有高亲和力结合的潜在候选物。并与其他结构相似的肺炎链球菌(SpCS)和结核分枝杆菌(MtCS)的CS进行了结合效力检测。序列和结构研究表明，LmCS与其他CS结构(1Q1L、1QXO、1R52、1R53、1SQ1、1UMO、1UMF、1ZTB、2011、2012、4ECD和2G85)相似，每个单体都呈现出具有中心螺旋核的β-α-β三明治结构。分子对接研究和ADME/Tox结果显示，ZINC03803450和ZINC20149031是结合LmCS活性位点最有效的分子。另外两个配体zinc13387711和ZINC16052528对LmCS、SpCS和MtCS三种结构均表现出较强的结合亲和力，与LmCS的结合预测抑制常数(K(i))分别为22.94 nM和35.84 nM。与先前报道的41种苯并呋喃-3[2H]- 1类似物相比，一种具有良好ADME/Tox性能和与SpCS的实验IC50 (nM)值为7000 nM的苯并呋喃-3[2H]- 1类似物CHEMBL135212也可以被认为是LmCS的潜在抑制剂。这些信息将有助于发现那些可能作为有效CS抑制剂的化合物。进一步的实验研究和构效关系的评估有助于开发潜在的李斯特菌病抑制剂，以及抗菌化疗。

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Structural analysis and molecular docking of potential ligands with chorismate synthase of Listeria monocytogenes: a novel antibacterial drug target.

Listeriosis, in particular that caused by Listeria monocytogenes, is a major foodborne pathogen, and its control is becoming difficult because of widespread emergence of drug resistance strains. Chorismate synthase (CS), an essential enzyme of shikimate pathway present only in bacteria, fungi, plant and some apicomplexan parasites, is a validated potential antimicrobial drug target. Antimicrobial development through the elucidation of essential structural features of the CS of L. monocytogenes (LmCS), identification and prioritization of potential lead compounds targeted against LmCS were done. Structure-based virtual screening and docking studies were performed using Autodock tools to retrieve potential candidates with high affinity binding against LmCS model from several ligand repositories. The potency of binding was also checked with other structurally similar CS from Streptococcus pneumoniae (SpCS) and Mycobacterium tuberculosis (MtCS). The sequence and structural studies revealed LmCS was similar to be other CS structures (1Q1L, 1QXO, 1R52, 1R53, 1SQ1, 1UMO, 1UMF, 1ZTB, 2011, 2012, 4ECD and 2G85) with each monomer presenting β-α-β sandwich topology with a central helical core. Molecular docking studies and ADME/Tox results revealed that ZINC03803450 and ZINC20149031 were most potent molecules binding into the active site of LmCS. Other two ligands ZINC13387711-and ZINC16052528 showed a strong binding affinity score against all three structures (LmCS, SpCS and MtCS) and bind to LmCS with the predicted inhibition constant (K(i)) values of 22.94 nM and 35.84 nM, respectively. A reported benzofuran-3[2H]-one analog CHEMBL135212 with good ADME/Tox properties and experimental IC50 (nM) value of 7000 nM with SpCS could also be considered as a potential inhibitor of LmCS, as compared to previously reported 41 benzofuran-3[2H]-one analogs against SpCS. This information will assist in discovering those compounds that may act as potent CS inhibitors. Further experimental studies and evaluation of structure-activity relationship could help in the development of potential inhibitors against listeriosis, as well as antibacterial chemotherapy.

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来源期刊

Indian journal of biochemistry & biophysics 生物-生化与分子生物学

CiteScore

2.90

自引率

50.00%

发文量

审稿时长

3 months

期刊介绍： Started in 1964, this journal publishes original research articles in the following areas: structure-function relationships of biomolecules; biomolecular recognition, protein-protein and protein-DNA interactions; gene-cloning, genetic engineering, genome analysis, gene targeting, gene expression, vectors, gene therapy; drug targeting, drug design; molecular basis of genetic diseases; conformational studies, computer simulation, novel DNA structures and their biological implications, protein folding; enzymes structure, catalytic mechanisms, regulation; membrane biochemistry, transport, ion channels, signal transduction, cell-cell communication, glycobiology; receptors, antigen-antibody binding, neurochemistry, ageing, apoptosis, cell cycle control; hormones, growth factors; oncogenes, host-virus interactions, viral assembly and structure; intermediary metabolism, molecular basis of disease processes, vitamins, coenzymes, carrier proteins, toxicology; plant and microbial biochemistry; surface forces, micelles and microemulsions, colloids, electrical phenomena, etc. in biological systems. Solicited peer reviewed articles on contemporary Themes and Methods in Biochemistry and Biophysics form an important feature of IJBB. Review articles on a current topic in the above fields are also considered. They must dwell more on research work done during the last couple of years in the field and authors should integrate their own work with that of others with acumen and authenticity, mere compilation of references by a third party is discouraged. While IJBB strongly promotes innovative novel research works for publication as full length papers, it also considers research data emanating from limited objectives, and extension of ongoing experimental works as ‘Notes’. IJBB follows “Double Blind Review process” where author names, affiliations and other correspondence details are removed to ensure fare evaluation. At the same time, reviewer names are not disclosed to authors.