Glennon J D, Sarkar B
Biochem J. 1982 Apr 1;203(1):15-23. doi: 10.1042/bj2030015.
Detailed studies are reported on the Ni(II)-binding site of human serum albumin (HSA) and the results are compared with those obtained from the N-terminal native-sequence peptide, l-aspartyl-l-alanyl-l-histidine N-methylamide (Asp-Ala-His-NHMe). Equilibrium dialysis of HSA and Ni(II) in 0.1m-N-ethylmorpholine/HCl buffer, pH 7.53, demonstrates a specific Ni(II)-binding site on the protein. l-Histidine, the low-molecular-weight Ni(II)-binding constituent of human serum, is shown to have a greater affinity for Ni(II) than does HSA. A small but significant amount of ternary complex HSA-Ni(II)-l-histidine is also present in the equilibrium mixture containing the three components. The log (association constant) values for the binary and ternary Ni(II) complexes are 9.57 and 16.23 respectively. The complex equilibria between Asp-Ala-His-NHMe and Ni(II) have been investigated by analytical potentiometry in aqueous solution (0.15m-NaCl, 25 degrees C). Several species, including MA, MA(2), MH(-2)A, and MH(-1)A(2) [where M and A represent Ni(II) ion and anionic peptide respectively], were detected in the system, MH(-2)A being the major complex species. Equilibrium studies involving Asp-Ala-His-NHMe, Ni(II) and l-histidine reveal the presence of a ternary complex MH(-1)AB (where B represents anionic l-histidine) at physiological pH. Detailed studies of visible-absorption spectra of HSA in the presence of Cu(II) and Ni(II) reveal that the two metal ions bind HSA at the same site. The visible-absorption spectrum of Ni(II)-HSA complex shows a highly absorbing peak at 420nm (epsilon(max.) = 137; with shoulder at 450-480nm) characteristic of a square planar or square pyramidal co-ordination arrangement about the metal ion. Similar visible-absorption characteristics were observed for the major species MH(-2)A in the Asp-Ala-His-NHMe-Ni(II) system (lambda(max.) = 420nm; epsilon(max.) = 135; with shoulder at 450-480nm). The combination of experimental results from the protein studies and the peptide analyses provides strong evidence for the structure of the Ni(II)-binding site of HSA as one that involves the alpha-amino nitrogen atom, two deprotonated peptide nitrogen atoms, the imidazole nitrogen atom and the side-chain carboxy group of the aspartic acid residue. On the basis of the results obtained from the individual ternary systems involving protein and peptide, a mechanism for the transportation of Ni(II) in the serum is proposed.
报道了关于人血清白蛋白(HSA)镍(II)结合位点的详细研究,并将结果与从N端天然序列肽L-天冬氨酰-L-丙氨酰-L-组氨酸N-甲酰胺(Asp-Ala-His-NHMe)获得的结果进行了比较。在pH 7.53的0.1m-N-乙基吗啉/盐酸缓冲液中对HSA和镍(II)进行平衡透析,证明该蛋白质上存在一个特定的镍(II)结合位点。L-组氨酸是人血清中低分子量的镍(II)结合成分,显示出对镍(II)的亲和力比HSA更高。在含有这三种成分的平衡混合物中也存在少量但显著量的三元复合物HSA-镍(II)-L-组氨酸。二元和三元镍(II)复合物的对数(缔合常数)值分别为9.57和16.23。通过分析电位滴定法在水溶液(0.15m-氯化钠,25℃)中研究了Asp-Ala-His-NHMe与镍(II)之间的络合物平衡。在该体系中检测到几种物种,包括MA、MA₂、MH⁻₂A和MH⁻₁A₂[其中M和A分别代表镍(II)离子和阴离子肽],MH⁻₂A是主要的络合物物种。涉及Asp-Ala-His-NHMe、镍(II)和L-组氨酸的平衡研究表明,在生理pH下存在三元复合物MH⁻₁AB(其中B代表阴离子L-组氨酸)。对在铜(II)和镍(II)存在下HSA的可见吸收光谱的详细研究表明,这两种金属离子在同一位点结合HSA。镍(II)-HSA复合物的可见吸收光谱在420nm处显示一个高吸收峰(εmax. = 137;在450 - 480nm处有肩峰),这是金属离子周围平面正方形或四方锥配位排列的特征。在Asp-Ala-His-NHMe - 镍(II)体系中,主要物种MH⁻₂A也观察到类似的可见吸收特征(λmax. = 420nm;εmax. = 135;在450 - 480nm处有肩峰)。蛋白质研究和肽分析的实验结果相结合,为HSA镍(II)结合位点的结构提供了有力证据,该结构涉及α-氨基氮原子、两个去质子化的肽氮原子、咪唑氮原子和天冬氨酸残基的侧链羧基。基于从涉及蛋白质和肽的各个三元体系获得的结果,提出了血清中镍(II)的转运机制。
