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与谷氨酸变位酶结合的腺苷钴胺素光解和重组的时间分辨测量。

Time-resolved measurements of the photolysis and recombination of adenosylcobalamin bound to glutamate mutase.

作者信息

Sension Roseanne J, Harris D Ahmasi, Stickrath Andrew, Cole Allwyn G, Fox Christel C, Marsh E Neil G

机构信息

Departments of Chemistry and of Physics, University of Michigan, Ann Arbor, Michigan 48109-1055, USA.

出版信息

J Phys Chem B. 2005 Sep 29;109(38):18146-52. doi: 10.1021/jp052492d.


DOI:10.1021/jp052492d
PMID:16853330
Abstract

Femtosecond to nanosecond transient absorption spectroscopy is used to investigate the photolysis of 5'-deoxyadenosylcobalamin (coenzyme B12, AdoCbl) bound to glutamate mutase. The photochemistry of AdoCbl is found to be inherently dependent upon the environment of the cofactor. Excitation of AdoCbl bound to glutamate mutase results in formation of a metal-to-ligand charge transfer intermediate state which decays to form cob(II)alamin with a time constant of 105 ps. This observation is in contrast to earlier measurements in water where the photohomolysis proceeds through an intermediate state in which the axial dimethylbenzimidazole ligand appears to have dissociated, and measurements in ethylene glycol where prompt bond homolysis is observed (Yoder, L. M.; Cole, A. G.; Walker, L. A., II; Sension, R. J. J. Phys. Chem. B 2001, 105, 12180-12188). The quantum yield for formation of stable radical pairs in the enzyme is found to be phi = 0.05 +/- 0.03, and the resulting intrinsic rate constants for geminate recombination and "cage escape" are 1.0 +/- 0.1 and 0.05 +/- 0.03 ns(-1), respectively. The rate constant for geminate recombination is 30% less than that observed for AdoCbl in water or ethylene glycol. This reduction is insufficient to account for the 10(12)-fold increase in the homolysis rate observed when substrate is bound to the protein. Finally, the protein provides a cage to prevent diffusive loss of the adenosyl radical; however, the ultimate yield for long-lived radicals is determined by the evolution from a singlet to a triplet radical pair as proposed for AdoCbl in ethylene glycol.

摘要

飞秒到纳秒瞬态吸收光谱法用于研究与谷氨酸变位酶结合的5'-脱氧腺苷钴胺素(辅酶B12,AdoCbl)的光解。发现AdoCbl的光化学本质上取决于辅因子的环境。与谷氨酸变位酶结合的AdoCbl的激发导致形成金属到配体的电荷转移中间态,该中间态以105皮秒的时间常数衰减形成钴胺素(II)(cob(II)alamin)。这一观察结果与早期在水中的测量结果形成对比,在水中光解通过轴向二甲基苯并咪唑配体似乎已经解离的中间态进行,也与在乙二醇中的测量结果不同,在乙二醇中观察到快速的键均裂(约德,L.M.;科尔,A.G.;沃克,L.A.,二世;森申,R.J.《物理化学杂志B》2001年,105卷,12180 - 12188页)。发现酶中稳定自由基对形成的量子产率为φ = 0.05 ± 0.03,并且由此产生的双分子复合和“笼逃逸”的固有速率常数分别为1.0 ± 0.1和0.05 ± 0.03纳秒⁻¹。双分子复合的速率常数比在水或乙二醇中观察到的AdoCbl的速率常数小30%。这种降低不足以解释当底物与蛋白质结合时观察到的均裂速率增加10¹²倍的现象。最后,蛋白质提供了一个笼以防止腺苷自由基的扩散损失;然而,长寿命自由基的最终产率由从单线态到三线态自由基对的演化决定,这与在乙二醇中对AdoCbl的提议相同。

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Time-resolved measurements of the photolysis and recombination of adenosylcobalamin bound to glutamate mutase.

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Visible-to-NIR-Light Activated Release: From Small Molecules to Nanomaterials.

Chem Rev. 2020-12-23

[2]
A New Facet of Vitamin B: Gene Regulation by Cobalamin-Based Photoreceptors.

Annu Rev Biochem. 2017-6-20

[3]
Beyond ferryl-mediated hydroxylation: 40 years of the rebound mechanism and C-H activation.

J Biol Inorg Chem. 2017-4

[4]
The photochemical mechanism of a B12-dependent photoreceptor protein.

Nat Commun. 2015-8-12

[5]
The Transcription Factor CarH Safeguards Use of Adenosylcobalamin as a Light Sensor by Altering the Photolysis Products.

Biochemistry. 2015-6-2

[6]
TD-DFT insight into photodissociation of the Co-C bond in coenzyme B12.

Front Chem. 2014-2-5

[7]
Entropic origin of cobalt-carbon bond cleavage catalysis in adenosylcobalamin-dependent ethanolamine ammonia-lyase.

J Am Chem Soc. 2013-10-1

[8]
Characterization of protein contributions to cobalt-carbon bond cleavage catalysis in adenosylcobalamin-dependent ethanolamine ammonia-lyase by using photolysis in the ternary complex.

J Am Chem Soc. 2011-4-14

[9]
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