Robinson N C, Zborowski J, Talbert L H
Department of Biochemistry, University of Texas Health Science Center, San Antonio 78284-7760.
Biochemistry. 1990 Sep 25;29(38):8962-9. doi: 10.1021/bi00490a012.
Detergent-solubilized bovine heart cytochrome c oxidase requires 2 mol of tightly bound cardiolipin (CL) per mole of monomeric complex for functional activity. Four lines of evidence support this conclusion: (1) Phospholipid depletion shows that two tightly bound CL's must remain associated with cytochrome c oxidase in order to maintain full electron transport activity. (2) Removal of the two tightly bound CL's correlates with decreased activity that is restored by reassociation of 2 mol of exogenous CL. (3) CL-depleted cytochrome c oxidase has two high-affinity binding sites for 2-[14C]acetylcardiolipin (AcCL), Kd,app less than 0.1 microM, that are not present in enzyme containing endogenous CL. An additional 2-3 lower affinity AcCL binding sites, Kd,app = 4 microM, are present in the CL-depleted complex, but these sites are also present in enzyme containing endogenous CL. (4) CL, monolysocardiolipin (MLCL), and dilysocardiolipin (DLCL) compete for AcCL binding with approximately the same relative affinities as those measured by the restoration of electron transport activity (MLCL competes much better than DLCL). However, MLCL and DLCL are only 60% and 15% as effective as CL in restoring maximum activity when they are bound to the high-affinity sites. The binding specificity of CL, MLCL, DLCL, and some of their acylated derivatives indicates that the apolar tails are most important for binding, not the polar head group. The presence or absence of hydroxyl groups in CL, MLCL, or DLCL also has little effect upon binding affinities. Binding specificity clearly favors CL since phosphatidylglycerol, phosphatidic acid, and phosphatidylcholine each have very low affinity for the CL binding sites (Kd,app greater than 20 microM). We, therefore, conclude that restoration of activity to CL-depleted cytochrome c oxidase is highly specific and requires the reassociation of CL, or structurally similar compounds, with two high-affinity binding sites.
经去污剂增溶的牛心细胞色素c氧化酶,每摩尔单体复合物需要2摩尔紧密结合的心磷脂(CL)才能发挥功能活性。有四条证据支持这一结论:(1)磷脂去除实验表明,必须有两个紧密结合的CL与细胞色素c氧化酶保持结合,才能维持完整的电子传递活性。(2)去除两个紧密结合的CL会导致活性降低,而重新结合2摩尔外源性CL可恢复活性。(3)CL耗尽的细胞色素c氧化酶对2-[14C]乙酰心磷脂(AcCL)有两个高亲和力结合位点,表观解离常数(Kd,app)小于0.1微摩尔,而含有内源性CL的酶中不存在这些位点。CL耗尽的复合物中还存在另外2 - 3个低亲和力的AcCL结合位点,Kd,app = 4微摩尔,但这些位点在含有内源性CL的酶中也存在。(4)CL、单赖氨酸心磷脂(MLCL)和双赖氨酸心磷脂(DLCL)竞争AcCL结合的相对亲和力与通过电子传递活性恢复所测得的亲和力大致相同(MLCL的竞争能力比DLCL强得多)。然而,当MLCL和DLCL与高亲和力位点结合时,它们恢复最大活性的效果仅为CL的60%和15%。CL、MLCL、DLCL及其一些酰化衍生物的结合特异性表明,非极性尾部对结合最为重要,而非极性头部基团。CL、MLCL或DLCL中羟基的存在与否对结合亲和力也几乎没有影响。结合特异性明显有利于CL,因为磷脂酰甘油、磷脂酸和磷脂酰胆碱对CL结合位点的亲和力都非常低(Kd,app大于20微摩尔)。因此,我们得出结论,使CL耗尽的细胞色素c氧化酶恢复活性具有高度特异性,需要CL或结构相似的化合物与两个高亲和力结合位点重新结合。
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