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作 者:李建辉[1] 吴伸[1] 姚宏兵[1] 邵鹏柱[1] 董贻诚
机构地区:[1]中国科学院生物物理研究所
出 处:《生物物理学报》1998年第4期589-594,共6页Acta Biophysica Sinica
基 金:国家自然科学基金;香港研究基金
摘 要:培养了(E160A)TCS和(E160D)TCS的单晶。在MARResearch面探测器系统上分别收集了0.193nm和0.20nm分辨率的X射线衍射数据。数据处理用MARSCALE程序系统完成。用同晶差值Fourier法解析了突变体的晶体结构,结构修正利用X-PLOR程序。修正结果,晶体学R因子分别为0.175,0.179,键长和键角的RMS偏差分别为0.0011nm和2.457°,0.0013nm和2.675°。在这两个突变体的结构中均未见到Glu189侧链方向的改变。通过对(E160A)TCS和(E160D)TCS的结构比较,说明(E160D)TCS活性低于(E160A)TCS的原因:这可能是由于在(E160D)TCS中Tyr111和Tyr70的侧链都具有较大的运动性,使它们与腺嘌呤碱基的芳香堆垛作用减弱。Crystals of (E160A)TCS and (E160D)TCS were grown by vapor diffusion method. X-ray diffraction data were collected to 0.193nm and 0.20nm resolution on a Mar Research area detector. The Mar Scale program was used for data processing and X-PLOR package. The structure analysis and their refinement were studied using Difference Fourier Method. The final crystallographic R factor is 0.175 and 0.179 respectively. The RMS deviations of bond length and angle of these mutants are 0.0011nm and 2.457, 0.0013nm and 2.675° respectively. The direction change of Glu189 side chain was not observed in these two crystal structures. The fact, that the activity of (E160D)TCS is less than (E160A)TCS, is elucidated by structure comparison .In (E160D)TCS structure the aromatic stack between Tyr111, Tyr70 and adenine is reduced because the movement of Tyr111 and Tyr70 side chain increase.
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