Duke E M, Wakatsuki S, Hadfield A, Johnson L N
Laboratory of Molecular Biophysics, University of Oxford, United Kingdom.
Protein Sci. 1994 Aug;3(8):1178-96. doi: 10.1002/pro.5560030804.
The conversion of substrate, heptenitol, to product, beta-1-C-methyl, alpha-D-glucose-1-phosphate (heptulose-2-P), in crystals of glycogen phosphorylase b has been studied by Laue and monochromatic diffraction methods. The phosphorolysis reaction in the crystal was started following liberation of phosphate from a caged phosphate compound, 3,5-dinitrophenyl phosphate (DNPP). The photolysis of DNPP, stimulated by flashes from a xenon flash lamp, was monitored in the crystal with a diode array spectrophotometer. In the Laue diffraction experiments, data to 2.8 A resolution were collected and the first time shot was obtained at 3 min from the start of reaction, and data collection comprised three 800-ms exposures. Careful data processing of Laue photographs for the large enzyme resulted in electron density maps of almost comparable quality to those produced by monochromatic methods. The difference maps obtained from the Laue measurements showed that very little catalysis had occurred 3 min and 1 h after release of phosphate, and a distinct peak consistent with the position expected for phosphate, in the attacking position was observed. Data collection times with monochromatic crystallographic methods on a home source took 16 h for data to 2.3 A resolution. Sufficient phosphate was released from the caged phosphate in the crystal from 5 flashes with a xenon flashlamp within 1 min for the reaction to go to completion within the time scale of the monochromatic data collection procedures. The heptulose-2-P product complex has been refined and the model agrees with that obtained previously with the major difference that the interchange of an aspartic acid (Asp 283) by an arginine (Arg 569) was not observed at the catalytic site. This change is part of the activation process of glycogen phosphorylase and may not have taken place in the current experiments because the caged compound binds weakly at the inhibitor site, restricting conformational change, and because activators of the enzymic reaction were not present in the crystal. In experiments with monochromatic radiation in which low phosphate concentrations were generated either by fewer photons or by diffusion of known phosphate concentrations, mixtures of substrate and product were observed. It was not possible through crystallographic refinement at 2.3 A resolution to establish the fractional occupancies of the enzyme-substrate and enzyme-product complexes, but the results did indicate that the reaction was proceeding slowly, consistent with approximate calculations for the likely rate of the reaction in the crystal.(ABSTRACT TRUNCATED AT 250 WORDS)
利用劳埃法和单色衍射法研究了糖原磷酸化酶b晶体中底物庚烯醇向产物β-1-C-甲基-α-D-葡萄糖-1-磷酸(庚酮糖-2-磷酸)的转化过程。晶体中的磷酸解反应是在笼形磷酸化合物3,5-二硝基苯磷酸酯(DNPP)释放出磷酸后开始的。用氙闪光灯的闪光刺激DNPP的光解,并通过二极管阵列分光光度计在晶体中进行监测。在劳埃衍射实验中,收集了分辨率为2.8 Å的数据,反应开始3分钟时获得了首张拍摄图像,数据收集包括三次800毫秒的曝光。对这种大型酶的劳埃照片进行仔细的数据处理后,得到的电子密度图质量几乎与单色法产生的图相当。从劳埃测量获得的差值图显示,在磷酸释放后3分钟和1小时,几乎没有发生催化作用,并且在进攻位置观察到一个与预期的磷酸位置一致的明显峰。在家用光源上用单色晶体学方法收集分辨率为2.3 Å的数据需要16小时。用氙闪光灯进行5次闪光,在1分钟内从晶体中的笼形磷酸中释放出足够的磷酸,使反应在单色数据收集程序的时间范围内完成。对庚酮糖-2-磷酸产物复合物进行了精修,模型与之前获得的模型一致,主要区别在于在催化位点未观察到天冬氨酸(Asp 283)被精氨酸(Arg 569)取代。这种变化是糖原磷酸化酶激活过程的一部分,在当前实验中可能没有发生,因为笼形化合物在抑制剂位点结合较弱,限制了构象变化,并且晶体中不存在酶促反应的激活剂。在使用单色辐射的实验中,通过较少的光子或已知磷酸浓度的扩散产生低磷酸浓度时,观察到了底物和产物的混合物。通过2.3 Å分辨率的晶体学精修无法确定酶-底物和酶-产物复合物的占有率,但结果确实表明反应进行缓慢,这与晶体中反应可能速率的近似计算结果一致。(摘要截短至250字)
