Finzel B C, Poulos T L, Kraut J
J Biol Chem. 1984 Nov 10;259(21):13027-36.
The crystal structure of cytochrome c peroxidase (EC 1.11.1.5) has been refined to an R factor of 0.20 computed for all reflections to 1.7 A. The refined molecular model includes 263 bound water molecules and allows for x-ray scattering by amorphous solvent. The mean positional error in atomic coordinates is estimated to lie between 0.12 and 0.21 A. Two factors are identified which may account for the ability of the enzyme to stabilize high-oxidation states of the heme iron during catalysis: 1) the proximal histidine forms a hydrogen bond with a buried aspartic acid side chain, Asp-235; and 2) the heme environment is more polar than in the cytochromes c or globins, owing to the presence of the partially buried side-chain of Arg-48 and five water molecules bound in close proximity to the heme. Two of these occupy the presumed peroxide-binding site. Two candidates are likely for the side chain that is oxidized to a free radical during formation of Compound I: 1) Trp-51, which rests 3.3 A above the heme plane in close proximity (2.7 A) to the sixth coordination position; and 2) Met-172, which is 3.7 A from the heme. Nucleophilic stabilization of the methionyl cation radical may be possible via Asp-235. His-181 is found to lie coplanar with the heme in a niche between the two propionates near the suspected cytochrome c-binding site. A network of hydrogen bonds involving this histidine may provide a preferred pathway for electron transfer between hemes.
细胞色素c过氧化物酶(EC 1.11.1.5)的晶体结构已被精修,对所有1.7 Å的反射计算得到的R因子为0.20。精修后的分子模型包括263个结合水分子,并考虑了无定形溶剂的X射线散射。原子坐标的平均位置误差估计在0.12至0.21 Å之间。确定了两个可能解释该酶在催化过程中稳定血红素铁高氧化态能力的因素:1)近端组氨酸与一个埋藏的天冬氨酸侧链Asp-235形成氢键;2)由于存在部分埋藏的Arg-48侧链和五个紧邻血红素结合的水分子,血红素环境比细胞色素c或球蛋白中的更具极性。其中两个水分子占据了假定的过氧化物结合位点。在化合物I形成过程中被氧化成自由基的侧链可能有两个候选者:1)Trp-51,它位于血红素平面上方3.3 Å处,紧邻第六配位位置(2.7 Å);2)Met-172,它距离血红素3.7 Å。天冬氨酸-235可能对甲硫氨酰阳离子自由基进行亲核稳定。发现His-181与血红素共面,位于疑似细胞色素c结合位点附近两个丙酸酯之间的一个壁龛中。涉及该组氨酸的氢键网络可能为血红素之间的电子转移提供一条优选途径。
