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β146组氨酸残基在血红蛋白玻尔效应分子基础中的作用:一项质子核磁共振研究。

Roles of the beta 146 histidyl residue in the molecular basis of the Bohr effect of hemoglobin: a proton nuclear magnetic resonance study.

作者信息

Busch M R, Mace J E, Ho N T, Ho C

机构信息

Department of Biological Sciences, Carnegie Mellon University, Pittsburgh, Pennsylvania 15213.

出版信息

Biochemistry. 1991 Feb 19;30(7):1865-77. doi: 10.1021/bi00221a020.

Abstract

Assessment of the roles of the carboxyl-terminal beta 146 histidyl residues in the alkaline Bohr effect in human normal adult hemoglobin by high-resolution proton nuclear magnetic resonance spectroscopy requires assignment of the resonances corresponding to these residues. Previous resonance assignments in low ionic strength buffers for the beta 146 histidyl residue in the carbonmonoxy form of hemoglobin have been controversial [see Ho and Russu (1987) Biochemistry 26, 6299-6305; and references therein]. By a careful spectroscopic study of human normal adult hemoglobin, enzymatically prepared des(His146 beta)-hemoglobin, and the mutant hemoglobins Cowtown (beta 146His----Leu) and York (beta 146His----Pro), we have resolved some of these conflicting results. By a close incremental variation of pH over a wide range in chloride-free 0.1 M N-(2-hydroxyethyl)piperazine-N'-2-ethanesulfonic acid buffer, a single resonance has been found to be consistently missing in the proton nuclear magnetic resonance spectra of these hemoglobin variants. The spectra of each of these variants show additional perturbations; therefore, the assignment has been confirmed by an incremental titration of buffer conditions to benchmark conditions, i.e., 0.2 M phosphate, where the assignment of this resonance is unambiguous. The strategy of incremental titration of buffer conditions also allows extension of this resonance assignment to spectra taken in 0.1 M [bis(2-hydroxyethyl)amino]tris(hydroxymethyl)methane buffer. Participation of the beta 146 histidyl residues in the Bohr effect has been calculated from the pK values determined for the assigned resonances in chloride-free 0.1 M N-(2-hydroxyethyl)piperazine-N'-2-ethanesulfonic acid buffer. Our results indicate that the contribution of the beta 146 histidyl residues is 0.52 H+/hemoglobin tetramer at pH 7.6, markedly less than the 0.8 H+/hemoglobin tetramer estimated by study of the mutant hemoglobin Cowtown (beta 146His----Leu) by Shih and Perutz [(1987) J. Mol. Biol. 195, 419-422]. We have found that at least two histidyl residues in the carbonmonoxy form of this mutant have pK values that are perturbed, and we suggest that these pK differences may in part account for this discrepancy. Furthermore, summation of the positive contribution of the beta 146 histidyl residues and the negative contribution of the beta 2 histidyl residues to the maximum Bohr effect measured in 0.1 M N-(2-hydroxyethyl)piperazine-N'-2-ethanesulfonic acid buffer suggests that additional sites in the hemoglobin molecule account for proton release upon ligation greater than the contribution of the beta 146 histidyl residues.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

通过高分辨率质子核磁共振光谱法评估羧基末端β146组氨酸残基在成人正常血红蛋白碱性玻尔效应中的作用,需要对与这些残基相对应的共振峰进行归属。先前在低离子强度缓冲液中对一氧化碳形式血红蛋白的β146组氨酸残基的共振峰归属一直存在争议[见Ho和Russu(1987年)《生物化学》26卷,6299 - 6305页;以及其中的参考文献]。通过对成人正常血红蛋白、酶法制备的去(His146β)-血红蛋白以及突变型血红蛋白考镇(β146His→Leu)和约克(β146His→Pro)进行仔细的光谱研究,我们解决了其中一些相互矛盾的结果。在无氯的0.1 M N -(2 - 羟乙基)哌嗪 - N'- 2 - 乙磺酸缓冲液中,通过在很宽的pH范围内进行紧密的增量变化,发现在这些血红蛋白变体的质子核磁共振光谱中始终缺少一个单一的共振峰。这些变体中每一个的光谱都显示出额外的扰动;因此,通过将缓冲条件逐步滴定至基准条件(即0.2 M磷酸盐,在此条件下该共振峰的归属是明确的),确认了该归属。缓冲条件的增量滴定策略还使得该共振峰归属能够扩展到在0.1 M [双(2 - 羟乙基)氨基]三(羟甲基)甲烷缓冲液中获得的光谱。根据在无氯的0.1 M N -(2 - 羟乙基)哌嗪 - N'- 2 - 乙磺酸缓冲液中为已归属共振峰测定的pK值,计算了β146组氨酸残基在玻尔效应中的参与情况。我们的结果表明,在pH 7.6时,β146组氨酸残基的贡献为0.52 H⁺/血红蛋白四聚体,明显小于Shih和Perutz通过对突变型血红蛋白考镇(β146His→Leu)的研究估计的0.8 H⁺/血红蛋白四聚体[(1987年)《分子生物学杂志》195卷,419 - 422页]。我们发现该突变体的一氧化碳形式中至少有两个组氨酸残基的pK值受到扰动,我们认为这些pK差异可能部分解释了这种差异。此外,在0.1 M N -(2 - 羟乙基)哌嗪 - N'- 2 - 乙磺酸缓冲液中测量的β146组氨酸残基的正贡献与β2组氨酸残基的负贡献之和表明,血红蛋白分子中的其他位点对结合时质子释放的贡献大于β146组氨酸残基的贡献。(摘要截短至400字)

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