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纳秒时间分辨荧光圆偏振:与马肝醇脱氢酶结合的烟酰胺腺嘌呤二核苷酸(NADH)的研究

Nanosecond time-resolved circular polarization of fluorescence: study of NADH bound to horse liver alcohol dehydrogenase.

作者信息

Schauerte J A, Schlyer B D, Steel D G, Gafni A

机构信息

Institute of Gerontology, University of Michigan, Ann Arbor 48109.

出版信息

Proc Natl Acad Sci U S A. 1995 Jan 17;92(2):569-73. doi: 10.1073/pnas.92.2.569.

Abstract

Circularly polarized luminescence (CPL) spectroscopy provides information on the excited-state chirality of a lumiphore analogous but complementary to information regarding the ground-state chirality derived from circular dichroism. The sensitivity of CPL spectra to molecular conformation makes this technique uniquely suited for the study of biomolecular structure, as extensively demonstrated in earlier studies. Unfortunately, the CPL spectra of many biomolecules often contain significantly overlapping contributions from emitting species either because multiple lumiphores are present (e.g., tryptophan residues in a protein) or because multiple conformations of the biomolecule simultaneously exist, each with a unique CPL spectrum. Increased resolution between individual contributions to the CPL may be achieved by time-resolving this signal, thus taking advantage of the fact that, as a rule, each of the emitting species also has a characteristic decay time associated with its electronically excited state. In addition, the time resolution provides information regarding dynamics associated with the different chiral states of the system. The present study describes an instrument for the determination of time-resolved CPL (TR-CPL) with subnanosecond resolution and its application to several chiral systems. The technique was first demonstrated on a model system with a strong time-dependent CPL signal. Subsequently, the circularly polarized component in the fluorescence of reduced nicotinamide adenine dinucleotide (NADH) bound to liver alcohol dehydrogenase was time-resolved. The CPL of NADH in the binary enzyme-coenzyme complex is time-dependent, reflecting structural differences around the reduced nicotinamide possibly due to a dynamic restructuring. In contrast, the CPL of the coenzyme in the ternary complex formed with enzyme and the substrate analog isobutyramide is essentially time-independent, likely reflecting a more rigid binding domain. Since the linear polarization of the fluorescence of the two complexes did not show any local flexibility of the NADH chromophore, the excited-state conformational rearrangement of the binary complex indicates a subtle change in its interactions with group(s) in direct contact with it.

摘要

圆偏振发光(CPL)光谱提供了关于发光体激发态手性的信息,这与源自圆二色性的基态手性信息类似但互补。CPL光谱对分子构象的敏感性使得该技术特别适合用于生物分子结构的研究,正如早期研究中广泛证明的那样。不幸的是,许多生物分子的CPL光谱往往包含来自发射物种的显著重叠贡献,这要么是因为存在多个发光体(例如蛋白质中的色氨酸残基),要么是因为生物分子同时存在多种构象,每种构象都有独特的CPL光谱。通过对该信号进行时间分辨,可以提高对CPL中各个贡献的分辨率,从而利用这样一个事实,即通常每个发射物种也有与其电子激发态相关的特征衰减时间。此外,时间分辨率提供了与系统不同手性状态相关的动力学信息。本研究描述了一种用于测定具有亚纳秒分辨率的时间分辨CPL(TR-CPL)的仪器及其在几个手性系统中的应用。该技术首先在具有强烈时间依赖性CPL信号的模型系统上得到验证。随后,对与肝醇脱氢酶结合的还原型烟酰胺腺嘌呤二核苷酸(NADH)荧光中的圆偏振成分进行了时间分辨。二元酶 - 辅酶复合物中NADH的CPL是时间依赖性的,反映了还原型烟酰胺周围的结构差异,这可能是由于动态重组所致。相比之下,与酶和底物类似物异丁酰胺形成的三元复合物中辅酶的CPL基本上与时间无关,这可能反映了一个更刚性的结合域。由于两种复合物荧光的线性偏振没有显示出NADH发色团的任何局部灵活性,二元复合物的激发态构象重排表明其与直接接触的基团之间的相互作用发生了细微变化。

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ZINC, A COMPONENT OF YEAST ALCOHOL DEHYDROGENASE.锌,酵母乙醇脱氢酶的一种成分。
Proc Natl Acad Sci U S A. 1955 Jun 15;41(6):327-38. doi: 10.1073/pnas.41.6.327.
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Methods Enzymol. 1978;49:179-99. doi: 10.1016/s0076-6879(78)49009-3.

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