Department of Chemistry, Northwestern University, 2145 Sheridan Road, Evanston, IL 60208-3113, USA.
Science. 2010 Nov 19;330(6007):1075-8. doi: 10.1126/science.1197054.
Direct measurements of electron transfer (ET) within a protein-protein complex with a redesigned interface formed by physiological partner proteins myoglobin (Mb) and cytochrome b(5) (b(5)) reveal interprotein ET rates comparable to those observed within the photosynthetic reaction center. Brownian dynamics simulations show that Mb in which three surface acid residues are mutated to lysine binds b(5) in an ensemble of configurations distributed around a reactive most-probable structure. Correspondingly, charge-separation ET from a photoexcited singlet zinc porphyrin incorporated within Mb to the heme of b(5) and the follow-up charge-recombination exhibit distributed kinetics, with median rate constants, k(f)(s) = 2.1 × 10(9) second(-1) and k(b)(s) = 4.3 × 10(10) second(-1), respectively. The latter approaches that for the initial step in photosynthetic charge separation, k = 3.3 × 10(11) second(-1).
直接测量蛋白质-蛋白质复合物内的电子转移(ET),该复合物由生理伴侣蛋白肌红蛋白(Mb)和细胞色素 b(5)(b(5))形成重新设计的界面,揭示了与光合作用反应中心内观察到的相当的蛋白间 ET 速率。布朗动力学模拟表明,Mb 中三个表面酸性残基突变为赖氨酸,与 b(5)结合形成围绕反应最可能结构分布的构象集合。相应地,从掺入 Mb 中的锌卟啉的光激发单线态到 b(5)的血红素的电荷分离 ET 和随后的电荷复合表现出分布动力学,中位速率常数 k(f)(s)=2.1×10(9)秒(-1)和 k(b)(s)=4.3×10(10)秒(-1),分别。后者接近光合作用电荷分离的初始步骤,k=3.3×10(11)秒(-1)。