Penning Trevor M
Center of Excellence in Environmental Toxicology, Department of Systems Pharmacology and Translational Therapeutics, Perelman School of Medicine, University of Pennsylvania, Philadelphia, PA 19104-6160, United States.
J Steroid Biochem Mol Biol. 2016 Jul;161:5-12. doi: 10.1016/j.jsbmb.2015.10.016. Epub 2015 Oct 24.
Structure-function studies on steroid transforming enzymes often use site-directed mutagenesis to inform mechanisms of catalysis and effects on steroid binding, and data are reported in terms of changes in steady state kinetic parameters kcat, Km and kcat/Km. However, this dissection of function is limited since kcat is governed by the rate-determining step and Km is a complex macroscopic kinetic constant. Often site-directed mutagenesis can lead to a change in the rate-determining step which cannot be revealed by just reporting a decrease in kcat alone. These issues are made more complex when it is considered that many steroid transforming enzymes have more than one substrate and product. We present the case for using transient-kinetics performed with stopped-flow spectrometry to assign rate constants to discrete steps in these multi-substrate reactions and their use to interpret enzyme mechanism and the effects of disease and engineered mutations. We demonstrate that fluorescence kinetic transients can be used to measure ligand binding that may be accompanied by isomerization steps, revealing the existence of new enzyme intermediates. We also demonstrate that single-turnover reactions can provide a klim for the chemical step and Ks for steroid-substrate binding and that when coupled with kinetic isotope effect measurements can provide information on transition state intermediates. We also demonstrate how multiple turnover experiments can provide evidence for either "burst-phase" kinetics, which can reveal a slow product release step, or linear-phase kinetics, in which the chemical step can be rate-determining. With these assignments it becomes more straightforward to analyze the effects of mutations. We use examples from the hydroxysteroid dehydrogenases (AKR1Cs) and human steroid 5β-reductase (AKR1D1) to illustrate the utility of the approach, which are members of the aldo-keto reductase (AKR) superfamily.
类固醇转化酶的结构-功能研究通常采用定点诱变来阐明催化机制及其对类固醇结合的影响,所报告的数据以稳态动力学参数kcat、Km和kcat/Km的变化形式呈现。然而,这种功能剖析存在局限性,因为kcat受速率决定步骤的支配,而Km是一个复杂的宏观动力学常数。定点诱变常常会导致速率决定步骤发生变化,而仅报告kcat的降低并不能揭示这一点。当考虑到许多类固醇转化酶具有不止一种底物和产物时,这些问题会变得更加复杂。我们阐述了使用停流光谱法进行瞬态动力学研究的理由,以便为这些多底物反应中的离散步骤确定速率常数,并利用这些常数来解释酶的作用机制以及疾病和工程突变的影响。我们证明荧光动力学瞬变可用于测量可能伴随异构化步骤的配体结合,从而揭示新的酶中间体的存在。我们还证明单周转反应可以为化学步骤提供一个klim,为类固醇底物结合提供一个Ks,并且当与动力学同位素效应测量相结合时,可以提供有关过渡态中间体的信息。我们还展示了多周转实验如何能够为“爆发相”动力学(可揭示缓慢的产物释放步骤)或线性相动力学(其中化学步骤可能是速率决定步骤)提供证据。通过这些赋值,分析突变的影响变得更加直接。我们以羟基类固醇脱氢酶(AKR1Cs)和人类固醇5β-还原酶(AKR1D1)为例来说明该方法的实用性,它们都是醛酮还原酶(AKR)超家族的成员。