Kimura Yukihiro, Hasegawa Koji, Ono Taka-aki
Laboratory for Photo-Biology, RIKEN Photodynamics Research Center, The Institute of Physical and Chemical Research, 519-1399 Aoba, Aramaki, Aoba, Sendai 980-0845, Japan.
Biochemistry. 2002 May 7;41(18):5844-53. doi: 10.1021/bi016093u.
Effects of Ca2+ depletion and substitution with other metal cations on the structure of the protein matrices of the oxygen-evolving complex (OEC) and their corresponding changes upon the S1 to S2 transition were examined using Fourier transform infrared (FTIR) spectroscopy. Ca2+ depletion and further supplementation with Li+, Na+, Mg2+, Ca2+, or Sr2+ did not significantly affect the typical vibrational features in the double difference S2/S1 spectrum, including the symmetric [1365(+)/1404(-) cm(-1)] and the asymmetric [1587(+)/1566(-) cm(-1)] stretching modes of the carboxylate ligand and the amide I and II modes of the backbone polypeptides. On the other hand, supplementation with K+, Rb+, Cs+, or Ba2+ significantly modified the S2/S1 spectrum, in which the carboxylate modes disappeared and the amide I and II modes were modified. Results indicate that the binding of metal cations that have ionic radii larger than that of Ca2+ to the Ca2+ site induces perturbations in the protein matrices in the vicinity of the Mn cluster to interrupt the characteristic structural and/or conformational changes upon the oxidation of the Mn cluster accompanied with the S1 to S2 transition. The spectrum was also altered by the supplementation of Cd2+, which has an ionic radius comparable to that of Ca2+. A single-pulse-induced S2/S1 difference spectrum revealed that bands that have been assigned to the vibrational modes for the Y(Z) tyrosine and the histidine ligand for the Mn cluster were not induced in the K+-supplemented membranes, although the histidine band is likely to be preserved in the Ca2+-depleted membranes. The Y(Z) band was considerably small in the double difference S2/S1 spectrum in the Ca2+-depleted and the cation-substituted membranes but distinctively present in the Sr2+- or Ca2+-replenished membranes. Furthermore, cation supplementation induced several new bands that disappeared following the Ca2+ replenishment. These results suggest that the proper organization of the hydrogen bond network within OEC for the water oxidation chemistry requires the Ca2+ ion and indicate that the role of Ca2+ is not purely structurally defined by the physical properties of the ion, such as valence and ionic radius. On the basis of these and other findings, we propose that Ca2+ is necessary for the formation of the hydrogen bond network that is involved in the reaction step of water oxidation.
利用傅里叶变换红外(FTIR)光谱研究了Ca2+耗尽以及用其他金属阳离子替代对析氧复合物(OEC)蛋白质基质结构的影响,以及它们在S1到S2转变时的相应变化。Ca2+耗尽以及进一步用Li+、Na+、Mg2+、Ca2+或Sr2+补充,对双差S2/S1光谱中的典型振动特征没有显著影响,包括羧酸盐配体的对称[1365(+)/1404(-) cm(-1)]和不对称[1587(+)/1566(-) cm(-1)]伸缩模式以及主链多肽的酰胺I和酰胺II模式。另一方面,用K+、Rb+、Cs+或Ba2+补充显著改变了S2/S1光谱,其中羧酸盐模式消失,酰胺I和酰胺II模式发生改变。结果表明,离子半径大于Ca2+的金属阳离子与Ca2+位点结合会在Mn簇附近的蛋白质基质中引起扰动,从而中断伴随S1到S2转变的Mn簇氧化时的特征结构和/或构象变化。补充具有与Ca2+相当离子半径的Cd2+也会改变光谱。单脉冲诱导的S2/S1差谱显示,在K+补充的膜中,未诱导出已被指定为Y(Z)酪氨酸和Mn簇组氨酸配体振动模式的谱带,尽管在Ca2+耗尽的膜中组氨酸谱带可能保留。在Ca2+耗尽和阳离子取代的膜中,双差S2/S1光谱中的Y(Z)谱带相当小,但在Sr2+或Ca2+补充的膜中明显存在。此外,阳离子补充诱导了几个新谱带,在Ca2+补充后消失。这些结果表明,OEC内水氧化化学反应的氢键网络的适当组织需要Ca2+离子,并表明Ca2+的作用并非纯粹由离子的物理性质(如化合价和离子半径)在结构上定义。基于这些及其他发现,我们提出Ca2+对于参与水氧化反应步骤的氢键网络的形成是必要的。
