首页> 美国卫生研究院文献>Biophysical Journal >Role of the coordinating histidine in altering the mixed valency of Cu(A): an electron nuclear double resonance-electron paramagnetic resonance investigation.
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Role of the coordinating histidine in altering the mixed valency of Cu(A): an electron nuclear double resonance-electron paramagnetic resonance investigation.

机译:组氨酸在改变铜(A)混合价中的作用:电子核双共振-电子顺磁共振研究。

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摘要

The binuclear Cu(A) site engineered into Pseudomonas aeruginosa azurin has provided a Cu(A)-azurin with a well-defined crystal structure and a CuSSCu core having two equatorial histidine ligands, His120 and His46. The mutations His120Asn and His120Gly were made at the equatorial His120 ligand to understand the histidine-related modulation to Cu(A), notably to the valence delocalization over the CuSSCu core. For these His120 mutants Q-band electron nuclear double resonance (ENDOR) and multifrequency electron paramagnetic resonance (EPR) (X, C, and S-band), all carried out under comparable cryogenic conditions, have provided markedly different electronic measures of the mutation-induced change. Q-band ENDOR of cysteine C(beta) protons, of weakly dipolar-coupled protons, and of the remaining His46 nitrogen ligand provided hyperfine couplings that were like those of other binuclear mixed-valence Cu(A) systems and were essentially unperturbed by the mutation at His120. The ENDOR findings imply that the Cu(A) core electronic structure remains unchanged by the His120 mutation. On the other hand, multifrequency EPR indicated that the H120N and H120G mutations had changed the EPR hyperfine signature from a 7-line to a 4-line pattern, consistent with trapped-valence, Type 1 mononuclear copper. The multifrequency EPR data imply that the electron spin had become localized on one copper by the His120 mutation. To reconcile the EPR and ENDOR findings for the His120 mutants requires that either: if valence localization to one copper has occurred, the spin density on the cysteine sulfurs and the remaining histidine (His46) must remain as it was for a delocalized binuclear Cu(A) center, or if valence delocalization persists, the hyperfine coupling for one copper must markedly diminish while the overall spin distribution on the CuSSCu core is preserved.
机译:工程化到铜绿假单胞菌天青中的双核Cu(A)位点提供了具有明确晶体结构的Cu(A)-天青素和具有两个赤道组氨酸配体His120和His46的CuSSCu核。突变His120Asn和His120Gly是在赤道His120配体上进行的,以了解组氨酸对Cu(A)的调节,特别是对CuSSCu核心上价键的离域化。对于这些His120突变体,在可比的低温条件下进行的Q波段电子核双共振(ENDOR)和多频电子顺磁共振(EPR)(X,C和S波段)提供了明显不同的突变电子手段引起的变化。半胱氨酸Cβ质子,弱偶极耦合质子和其余His46氮配体的Q带ENDOR提供了超精细的耦合,这与其他双核混合价Cu(A)系统的耦合一样,并且基本上不受干扰。 His120发生突变。 ENDOR的发现表明,His120突变使Cu(A)核心电子结构保持不变。另一方面,多频EPR表明H120N和H120G突变已将EPR超精细特征从7线变为4线,与捕获价1型单核铜一致。多频EPR数据表明,由于His120突变,电子自旋已定位在一根铜上。要调和His120突变体的EPR和ENDOR结果,需要采取以下两种方法之一:如果价位定位在一根铜上,则半胱氨酸硫和其余组氨酸(His46)的自旋密度必须保持不变,就象离域的双核Cu(A)一样。 )中心,或者如果化合价持续存在,则必须保留一种铜的超精细耦合,同时保留CuSSCu核上的整体自旋分布。

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