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辣根过氧化物酶同工酶的质子核磁共振光谱:独特光谱与同工酶比活性的相关性

Proton nuclear magnetic resonance spectroscopy of horseradish peroxidase isoenzymes: correlation of distinctive spectra with isoenzyme specific activities.

作者信息

Gonzalez-Vergara E, Meyer M, Goff H M

出版信息

Biochemistry. 1985 Nov 5;24(23):6561-7. doi: 10.1021/bi00344a038.

DOI:10.1021/bi00344a038
PMID:4084538
Abstract

High-resolution proton NMR spectra are reported for the paramagnetic ferric native and cyano complexes of the five major horseradish root peroxidase (HRP) isoenzymes (A1, A2, A3, B, and C). Axial imidazole resonances are observed in the native and cyano-complex spectra of all the isoenzymes, thus indicating the presence of a common axial histidine ligand. Proton NMR spectra outside the usual diamagnetic region are identical for sets of A1 and A2 isoenzymes and for the B and C isoenzyme set. Variation in heme residue chemical shift positions may be controlled in part by porphyrin vinyl side chain-protein interactions. Diverse upfield spectra among the isoenzymes reflect amino acid substitutions and/or conformational differences near the prosthetic group, as signals in this region must result from amino acid residues in proximity to the heme center. Acid-base dependence studies reveal an "alkaline" transition that converts the native high-spin iron (III) porphyrin to the low-spin state. The transition occurs at pH 9.3, 9.4, 9.8, and 10.9 for respective HRP A1, A2, A3, and C isoenzymes, respectively. Significantly, this ordering also reflects specific activities for the isoenzymes in the order A1 = A2 greater than A3 greater than B = C. Identical proton NMR spectra for A1/A2 and B/C isoenzyme sets parallel equivalent specific activities for members of a particular set. Proton NMR spectra thus appear to be highly sensitive to protein modifications that affect catalytic activity.

摘要

报道了五种主要辣根过氧化物酶(HRP)同工酶(A1、A2、A3、B和C)的顺磁性铁原生和氰基配合物的高分辨率质子核磁共振谱。在所有同工酶的原生和氰基配合物谱中均观察到轴向咪唑共振,因此表明存在共同的轴向组氨酸配体。A1和A2同工酶组以及B和C同工酶组在通常的抗磁性区域之外的质子核磁共振谱是相同的。血红素残基化学位移位置的变化可能部分受卟啉乙烯基侧链与蛋白质相互作用的控制。同工酶之间不同的高场谱反映了辅基附近的氨基酸取代和/或构象差异,因为该区域的信号必定来自靠近血红素中心的氨基酸残基。酸碱依赖性研究揭示了一种“碱性”转变,该转变将原生的高自旋铁(III)卟啉转变为低自旋状态。对于HRP A1、A2、A3和C同工酶,转变分别发生在pH 9.3、9.4、9.8和10.9。值得注意的是,这种排序也反映了同工酶的比活性顺序为A1 = A2大于A3大于B = C。A1/A2和B/C同工酶组相同的质子核磁共振谱与特定组中成员的等效比活性平行。因此,质子核磁共振谱似乎对影响催化活性的蛋白质修饰高度敏感。

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Proton nuclear magnetic resonance spectroscopy of horseradish peroxidase isoenzymes: correlation of distinctive spectra with isoenzyme specific activities.辣根过氧化物酶同工酶的质子核磁共振光谱:独特光谱与同工酶比活性的相关性
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