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铜(II)与tau 蛋白 R3 区八肽片段的结合特性:电位滴定、光谱和质谱联合研究。

Copper (II) binding properties of an octapeptide fragment from the R3 region of tau protein: A combined potentiometric, spectroscopic and mass spectrometric study.

机构信息

Department of Inorganic and Analytical Chemistry, University of Debrecen, Egyetem tér 1, H-4032 Debrecen, Hungary.

CNR-Istituto di Cristallografia (IC), s.s. Catania, Via Paolo Gaifami 18, I-95126 Catania, Italy.

出版信息

J Inorg Biochem. 2021 Apr;217:111358. doi: 10.1016/j.jinorgbio.2021.111358. Epub 2021 Jan 28.

DOI:10.1016/j.jinorgbio.2021.111358
PMID:33588277
Abstract

The copper(II) complexes of a peptide fragment of the R3 domain of tau protein (tau(326-333) Ac-GNIHHKPG-NH) and its mutants (Ac-GNGHHKPG-NH, Ac-GNIHHKAG-NH, Ac-GNGAHKPG-NH and Ac-GNGHAKPG-NH) have been studied by potentiometric and spectroscopic (UV-Vis, CD) methods. ESR spectroscopy and mass spectrometry were also used to prove the coordination mode of the mononuclear complexes and the formation of dinuclear species, respectively. It has been demonstrated that the (326-333) fragment of tau protein is a versatile and effective ligand for copper(II) coordination. The versatility of copper(II) binding is related to the presence of two adjacent histidyl residues in the sequence, which results in the coexistence of mononuclear, bis(ligand) and dinuclear complexes at different metal to ligand ratios. The 1:1 mononuclear complexes are, however, the dominant species with all peptides and the imidazole-N and one to three deprotonated amide nitrogen atoms towards the N-terminal side of the histidyl residue have been suggested as metal binding sites. This binding mode allows the formation of coordination isomers because any of the two histidine moieties can be the primary anchoring site. It is evident from the CD spectroscopic measurements that the isomers are present in almost equal concentration. The copper(II) binding affinity of the native fragment of tau protein is comparable to that of a similar 2-histidine fragment of amyloid-β mutant, Ac-SGAEGHHQK-NH but the comparison with an independent histidyl residue (H32) from the N-terminal region of the protein reveals the predominance of H32 over the histidines in the R3 domain.

摘要

已通过电位法和光谱法(UV-Vis、CD)研究了微管相关蛋白 tau 蛋白的 R3 结构域肽片段(tau(326-333) Ac-GNIHHKPG-NH)及其突变体(Ac-GNGHHKPG-NH、Ac-GNIHHKAG-NH、Ac-GNGAHKPG-NH 和 Ac-GNGHAKPG-NH)的铜(II)配合物。ESR 光谱和质谱也分别用于证明单核配合物的配位模式和双核物种的形成。已证明,tau 蛋白的(326-333)片段是铜(II)配位的多功能有效配体。铜(II)结合的多功能性与序列中两个相邻组氨酸残基的存在有关,这导致在不同金属与配体比下存在单核、双(配体)和双核配合物。然而,1:1 单核配合物是所有肽的主要物种,并且咪唑-N 和一个至三个去质子酰胺氮原子朝向组氨酸残基的 N-末端被认为是金属结合位点。这种结合模式允许形成配位异构体,因为两个组氨酸部分中的任何一个都可以成为主要锚定位点。从 CD 光谱测量可以明显看出,几乎以相等的浓度存在异构体。天然tau 蛋白片段的铜(II)结合亲和力可与类似的淀粉样β突变体 Ac-SGAEGHHQK-NH 的 2-组氨酸片段相媲美,但与来自蛋白 N-末端区域的独立组氨酸(H32)的比较表明,H32 优先于 R3 结构域中的组氨酸。

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