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α-血红蛋白稳定蛋白 (AHSP) 显著降低了人 HbA 的 α-亚基与过氧化氢的氧化还原电位和反应活性。

α-Hemoglobin stabilizing protein (AHSP) markedly decreases the redox potential and reactivity of α-subunits of human HbA with hydrogen peroxide.

机构信息

Laboratory of Biochemistry and Vascular Biology, Division of Hematology, Center for Biologics Evaluation and Research, Food and Drug Administration, Bethesda, Maryland 20852, USA.

出版信息

J Biol Chem. 2013 Feb 8;288(6):4288-98. doi: 10.1074/jbc.M112.412064. Epub 2012 Dec 21.

Abstract

α-Hemoglobin stabilizing protein (AHSP) is a molecular chaperone that binds monomeric α-subunits of human hemoglobin A (HbA) and modulates heme iron oxidation and subunit folding states. Although AHSP·αHb complexes autoxidize more rapidly than HbA, the redox mechanisms appear to be similar. Both metHbA and isolated met-β-subunits undergo further oxidation in the presence of hydrogen peroxide (H(2)O(2)) to form ferryl heme species. Surprisingly, much lower levels of H(2)O(2)-induced ferryl heme are produced by free met-α-subunits as compared with met-β-subunits, and no ferryl heme is detected in H(2)O(2)-treated AHSP·met-α-complex at pH values from 5.0 to 9.0 at 23 °C. Ferryl heme species were similarly not detected in AHSP·met-α Pro-30 mutants known to exhibit different rates of autoxidation and hemin loss. EPR data suggest that protein-based radicals associated with the ferryl oxidation state exist within HbA α- and β-subunits. In contrast, treatment of free α-subunits with H(2)O(2) yields much smaller radical signals, and no radicals are detected when H(2)O(2) is added to AHSP·α-complexes. AHSP binding also dramatically reduces the redox potential of α-subunits, from +40 to -78 mV in 1 m glycine buffer, pH 6.0, at 8 °C, demonstrating independently that AHSP has a much higher affinity for Fe(III) versus Fe(II) α-subunits. Hexacoordination in the AHSP·met-α complex markedly decreases the rate of the initial H(2)O(2) reaction with iron and thus provides α-subunits protection against damaging oxidative reactions.

摘要

α-血红蛋白稳定蛋白(AHSP)是一种分子伴侣,可结合人血红蛋白 A(HbA)的单体α-亚基,并调节血红素铁氧化和亚基折叠状态。虽然 AHSP·αHb 复合物的自氧化速度比 HbA 更快,但氧化还原机制似乎相似。在过氧化氢(H₂O₂)存在下,MetHbA 和分离的 Met-β-亚基都进一步氧化,形成高铁血红素物种。令人惊讶的是,与 Met-β-亚基相比,游离 Met-α-亚基产生的 H₂O₂诱导的高铁血红素要低得多,并且在 pH 值为 5.0 至 9.0 的范围内,在 23°C 下,AHSP·met-α-复合物在 H₂O₂处理下未检测到高铁血红素。在 AHSP·met-α Pro-30 突变体中也未检测到高铁血红素物种,该突变体已知具有不同的自氧化和血红素损失速率。EPR 数据表明,与高铁氧化态相关的蛋白自由基存在于 HbA 的α-和β-亚基中。相比之下,用 H₂O₂处理游离的α-亚基会产生较小的自由基信号,并且当将 H₂O₂添加到 AHSP·α-复合物中时,未检测到自由基。AHSP 结合还极大地降低了α-亚基的氧化还原电位,从+40 降低至-78 mV,在 1 m 甘氨酸缓冲液,pH 值为 6.0,在 8°C,独立证明 AHSP 对 Fe(III)与 Fe(II)α-亚基的亲和力高得多。AHSP·met-α 复合物中的六配位显著降低了 H₂O₂与铁的初始反应速率,从而为α-亚基提供了对破坏性氧化反应的保护。

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