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Comparison of x-ray crystal structures of an acyl-enzyme intermediate of subtilisin Carlsberg formed in anhydrous acetonitrile and in water

机译:枯草杆菌蛋白酶嘉士伯在无水乙腈和水中形成的酰基酶中间体的X射线晶体结构比较

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摘要

The x-ray crystal structures of trans-cinnamoyl–subtilisin, an acyl-enzyme covalent intermediate of the serine protease subtilisin Carlsberg, have been determined to 2.2-Å resolution in anhydrous acetonitrile and in water. The cinnamoyl–subtilisin structures are virtually identical in the two solvents. In addition, their enzyme portions are nearly indistinguishable from previously determined structures of the free enzyme in acetonitrile and in water; thus, acylation in either aqueous or nonaqueous solvent causes no appreciable conformational changes. However, the locations of bound solvent molecules in the active site of the acyl- and free enzyme forms in acetonitrile and in water are distinct. Such differences in the active site solvation may contribute to the observed variations in enzymatic activities. On prolonged exposure to organic solvent or removal of interstitial solvent from the crystal lattice, the channels within enzyme crystals are shown to collapse, leading to a drop in the number of active sites accessible to the substrate. The mechanistic and preparative implications of our findings for enzymatic catalysis in organic solvents are discussed.
机译:在无水乙腈和水中,反式肉桂酰基枯草杆菌蛋白酶(丝氨酸蛋白酶枯草杆菌蛋白酶Carlsberg的一种酰基酶共价中间体)的X射线晶体结构已确定为2.2-Å分辨率。两种溶剂中的肉桂酰基-枯草杆菌蛋白酶结构几乎相同。此外,它们的酶部分与乙腈和水中游离酶的先前确定的结构几乎没有区别;因此,在水性或非水性溶剂中的酰化均不会引起明显的构象变化。但是,结合的溶剂分子在乙腈和水中的酰基和游离酶形式的活性部位的位置是不同的。活性位点溶剂化的这种差异可能有助于观察到的酶活性变化。在长时间暴露于有机溶剂或从晶格中除去间隙溶剂时,酶晶体内的通道显示塌陷,导致底物可及的活性位点数量减少。讨论了我们的发现对有机溶剂中酶催化作用的机理和制备意义。

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