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在抹香鲸高铁肌红蛋白与单当量过氧化氢的自氧化反应中,色氨酸-14是DBNBS自旋捕获的首选位点。

Tryptophan-14 is the preferred site of DBNBS spin trapping in the self-peroxidation reaction of sperm whale metmyoglobin with a single equivalent of hydrogen peroxide.

作者信息

Gunther Michael R, Tschirret-Guth Richard A, Lardinois Olivier M, Ortiz de Montellano Paul R

机构信息

Department of Biochemistry and Molecular Pharmacology, West Virginia University, Morgantown 26506, USA.

出版信息

Chem Res Toxicol. 2003 May;16(5):652-60. doi: 10.1021/tx0256580.

Abstract

The 3,5-dibromo-4-nitrosobenzenesulfonate (DBNBS)-metmyoglobin adduct formed following the horse metmyoglobin-H(2)O(2) reaction has been assigned to both a tyrosyl and a tryptophanyl residue radical. At low H(2)O(2), hyperfine coupling to a (13)C atom in sperm whale metmyoglobin labeled at the tryptophan residues with (13)C allowed the unequivocal assignment of the primary adduct to a tryptophanyl radical. Trapping at Trp-14 of sperm whale myoglobin was indicated by greatly decreased electron paramagnetic resonance (EPR) spectral intensity of the DBNBS adducts of the Trp-14-Phe recombinant proteins. Complex EPR spectra with partially resolved hyperfine splittings from several atoms were obtained by pronase treatment of the DBNBS/*W14F metmyoglobin adducts. The EPR spectra of authentic DBNBS/*Tyr adducts were incubation time-dependent; the late time spectra resembled the spectra of pronase-treated DBNBS/*W14F sperm whale myoglobin adducts, suggesting formation of an unstable tyrosyl radical adduct in the latter proteins. When the H(2)O(2):metmyoglobin ratio was increased to 5:1, the EPR spectrum after pronase treatment supported trapping of a tyrosyl radical, although similar decreases in tryptophan content were detected at H(2)O(2):metmyoglobin ratios of 1:1 and 5:1.

摘要

在马肌红蛋白与过氧化氢反应后形成的3,5-二溴-4-亚硝基苯磺酸盐(DBNBS)-高铁肌红蛋白加合物,已被确定与一个酪氨酸残基自由基和一个色氨酸残基自由基有关。在低过氧化氢浓度下,与用¹³C标记色氨酸残基的抹香鲸高铁肌红蛋白中的一个¹³C原子的超精细偶合,使得能够明确将主要加合物确定为色氨酸残基自由基。抹香鲸肌红蛋白Trp-14处的捕获通过Trp-14-Phe重组蛋白的DBNBS加合物的电子顺磁共振(EPR)光谱强度大幅降低得以表明。通过对DBNBS/*W14F高铁肌红蛋白加合物进行链霉蛋白酶处理,获得了具有来自几个原子的部分分辨超精细分裂的复杂EPR光谱。真实的DBNBS/*Tyr加合物的EPR光谱与孵育时间有关;后期光谱类似于链霉蛋白酶处理的DBNBS/*Wl4F抹香鲸肌红蛋白加合物的光谱,表明在后者蛋白质中形成了不稳定的酪氨酸残基自由基加合物。当过氧化氢与高铁肌红蛋白的比例增加到5:1时,链霉蛋白酶处理后的EPR光谱支持捕获酪氨酸残基自由基,尽管在过氧化氢与高铁肌红蛋白比例为1:1和5:1时检测到色氨酸含量有类似的降低。

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