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Choreographing an enzyme's dance

机译:编排酶的舞蹈

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While ground state structures combined with chemical tools and enzyme kinetics deliver useful information on possible chemical mechanisms of enzyme catalysis, they do not unravel the finely balanced energy inventory to explain the impressive rate enhancement of enzymes. For this goal, a complete description of enzyme catalysis in the form of an energy landscape is needed. Since the rate of catalysis is determined by the climb over a sequence of energy barriers, we focus here on the critical question of transition pathways. A combination of time-resolved NMR and simulation deliver a glimpse into how proteins can so efficiently move within the ensemble of the native conformations while avoiding unfolding during that journey. The loss of energy due to breakage of native contacts is compensated by non-native transient hydrogen bonds during the transition thereby 'holding on' to the energy until the new native contacts form that define the alternate functional state. The use of kinetic isotope effects (KIE) to study the chemical step show that coordinated atomic fluctuations of the protein component dictate the probability of 'correct' distance and orientation, due to its extreme sensitivity to distance. The examples here stress the point that highly choreographed conformational sampling together with chemical integrity is a prerequisite for efficient enzyme catalysis.
机译:尽管基态结构与化学工具和酶动力学相结合可提供有关酶催化可能的化学机理的有用信息,但它们并没有揭示精细平衡的能量库存,无法解释酶的惊人速率提高。为此,需要以能量分布图的形式完整描述酶催化作用。由于催化速率是由一系列能垒的爬升决定的,因此我们在此重点讨论过渡途径这一关键问题。时间分辨的NMR和模拟相结合,使人们可以一眼了解蛋白质如何在天然构象的整体内如此有效地运动,同时避免在此过程中展开。在过渡过程中,由于天然接触的破坏而造成的能量损失可以通过非天然的瞬态氢键得到补偿,从而“保持”能量直至形成新的天然接触,从而形成了交替的功能状态。利用动力学同位素效应(KIE)研究化学步骤表明,蛋白质组分的协调原子波动决定了“正确”的距离和方向的可能性,这是由于其对距离的极度敏感性。这里的例子强调了这一点,即高度编排的构象采样以及化学完整性是有效酶催化的先决条件。

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