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Nanoelectrospray Ionization Mass Spectrometric Study of Mycobacterium tuberculosis CYP121-Ligand Interactions

机译:结核分枝杆菌CYP121-配体相互作用的纳米电喷雾电离质谱研究

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Nondenaturing nanoelectrospray ionization mass spectrometry (nanoESI MS) of intact protein complexes was used to study CYP121, one of the 20 cytochrome P450s in Mycobacterium tuberculosis (Mtb) and an enzyme that is essential for bacterial viability. The results shed new light on both ligand-free and ligand-bound states of CYP121. Isolated unbound CYP121 is a predominantly dimeric protein, with a minor monomeric form present. High affinity azoles cause the dissociation of dimeric CYP121 into monomer, whereas weaker azole binders induce partial dimer dissociation or do not significantly destabilize the dimer. Complexes of CYP121 with azoles were poorly detected by nanoESI MS, indicating kinetically labile complexes that are easily prone to gas-phase dissociation. Unlike with the azoles, CYP121 forms a stable complex with its natural substrate cYY that does not undergo gas-phase dissociation. In addition, a series of potential ligands from fragment-based studies were used as a test for nanoESI MS work against CYP121. Most of these ligands formed stable complexes with CYP121, and their binding did not promote dimer dissociation. On the basis of binding to the monomer and/or CYP121 dimer it was possible to determine the relative order of their CYP121 binding affinities. The top nanoESI MS screening hit was confirmed by heme absorbance shift assay to have a K_d of 40 μM.
机译:完整蛋白复合物的非变性纳米电喷雾电离质谱法(nanoESI MS)用于研究CYP121,它是结核分枝杆菌(Mtb)中20种细胞色素P450之一,并且是细菌生存力所必需的酶。结果为CYP121的无配体和配体结合状态提供了新的启示。分离的未结合的CYP121是主要的二聚体蛋白,具有次要的单体形式。高亲和力的唑类导致二聚体CYP121分解为单体,而较弱的唑类结合剂则引起部分二聚体解离或不会显着破坏二聚体的稳定性。 nanoESI MS很难检测到CYP121与吡咯的复合物,表明动力学不稳定的复合物很容易发生气相离解。与唑类不同,CYP121与它的天然底物cYY形成稳定的复合物,而不会发生气相离解。此外,来自片段研究的一系列潜在配体被用作nanoESI MS针对CYP121的测试。这些配体中的大多数与CYP121形成稳定的复合物,它们的结合没有促进二聚体的解离。基于与单体和/或CYP121二聚体的结合,可以确定它们的CYP121结合亲和力的相对顺序。通过血红素吸光度漂移测定法确认了最高的nanoESI MS筛选结果的K_d为40μM。

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