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Molecular modelling and docking studies of an α-1,4-amylase from endophytic Bacillus amyloliquefaciens

机译:内生解淀粉芽孢杆菌α-1,4-淀粉酶的分子模型和对接研究

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α-1,4-Amylase is one of the most important industrial enzymes and there is enormous interest in isolating α-1,4-amylase with better properties. The α-1,4-amylase producing endophytic Bacillus amyloliquefaciens was isolated and characterized from Hevea brasiliensis . The α-1,4-amylase gene after cloning and sequencing contained 1542 base pairs. A homology model of the α-1,4-amylase enzyme was built from the deduced amino acid sequence. The modelled and template α-1,4-amylase enzyme (PDB ID:3bh4) showed 97.7% sequence identity with similar secondary and tertiary structures. Computer aided docking studies of the substrate (maltotetraose) with the modelled as well as the template enzymes showed that although the binding energies were almost the same in both the complexes, the number of hydrogen bonds and van der Waals interactions in the active sites of the two enzymes were different. These variations might be due to the change in the amino acid residues of the active site regions of two enzymes. The mutated polar amino acids in the active site of modelled α-1,4-amylase favoured more hydrogen bond formation with the substrate. The difference in the active site interactions may improve the specificity of the enzyme and affect the catalytic potential of α-1,4-amylase.
机译:α-1,4-淀粉酶是最重要的工业酶之一,人们对分离具有更好性能的α-1,4-淀粉酶有着极大的兴趣。从巴西橡胶树中分离并鉴定了产生α-1,4-淀粉酶的内生解淀粉芽孢杆菌。克隆和测序后的α-1,4-淀粉酶基因包含1542个碱基对。由推导的氨基酸序列建立α-1,4-淀粉酶的同源性模型。建模和模板化的α-1,4-淀粉酶(PDB ID:3bh4)显示97.7%的序列同一性,具有相似的二级和三级结构。计算机辅助的底物(麦芽四糖)与模型酶和模板酶的对接研究表明,尽管两种复合物中的结合能几乎相同,但在活性位点中氢键的数量和范德华相互作用两种酶是不同的。这些变化可能是由于两种酶的活性位点区域的氨基酸残基的变化。模拟的α-1,4-淀粉酶活性位点中突变的极性氨基酸有利于与底物形成更多的氢键。活性位点相互作用的差异可能会提高酶的特异性,并影响α-1,4-淀粉酶的催化潜力。

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