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Dynamics of a mobile loop at the active site of Escherichia coli asparaginase

机译:大肠杆菌天冬酰胺酶活性位点移动环的动力学

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Asparaginase II from Escherichia coli is well-known member of the bacterial class II amidohydrolases. Enzymes of this family utilize a peculiar catalytic mechanism in which a pair of threonine residues play pivotal roles. Another common feature is a mobile surface loop that closes over the active site when the substrates is bound. We have studied the motion of the loop by stopped-flow experiments using the fluorescence of tryptophan residues as the spectroscopic probe. With wild-type enzyme the fluorescence of the only tryptophan, W66, was monitored. Here asparagine induced a rapid closure of the loop. The rate constants of the process (100-150 s~(-1) at 4℃) were considerably higher than those of the rate-limiting catalytic step. A more selective spectroscopic probe was generated by replacing W66 with tyrosine and Y25, a component of the loop, with tryptophan. In the resulting enzyme variant, k_(cat) and the rate of loop movement were reduced by factors of 10~2 and > 10~3, respectively, while substrate binding was unaffected. This indicates that the presence of tyrosine in position 25 is essential for both loop closure and catalysis. Numerical simulations of the observed transients are consistent with a model where loop closure is an absolute prerequisite for substrate turnover.
机译:来自大肠杆菌的天冬酰胺酶II是细菌II类酰胺水解酶的众所周知的成员。该家族的酶利用独特的催化机制,其中一对苏氨酸残基起关键作用。另一个共同的特点是可移动的表面环,当结合基材时,该表面环在活性部位上闭合。我们已经通过使用色氨酸残基的荧光作为光谱探针的停流实验研究了环路的运动。使用野生型酶,可以监测唯一的色氨酸W66的荧光。在此,天冬酰胺诱导环路的快速闭合。该工艺的速率常数(4℃时为100-150 s〜(-1))明显高于限速催化步骤的速率常数。通过将W66替换为酪氨酸,并将Y25(环路的一个组成部分)替换为色氨酸,从而生成了更具选择性的光谱探针。在所得的酶变体中,k_(cat)和环运动速率分别降低了10〜2和> 10〜3倍,而底物结合未受影响。这表明第25位酪氨酸的存在对于闭环和催化都是必不可少的。观察到的瞬态的数值模拟与模型相吻合,其中闭环是基板周转的绝对前提。

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