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Tryptophan dynamics of the FK506 binding protein: time-resolved fluorescence and simulations.

机译:FK506结合蛋白的色氨酸动力学:时间分辨荧光和模拟。

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摘要

The FK506-binding protein (FKBP12) is important in the immunosuppressant action of FK506 and rapamycin. We have investigated Trp side chain dynamics in FKBP12, with and without a bound immunosuppressant, by measuring the Trp time-resolved fluorescence anisotropy decay r(t). The r(t) for W59 in aqueous uncomplexed FKBP12 at 20 degrees C is well described by a single exponential with a recovered initial anisotropy, r(eff)o, of 0.192 and an overall rotational correlation time for the protein, phi p, of 4.7 ns; r(eff)o = 0.214 and phi p = 4.2 ns for the FKBP12/FK506 complex. Using an expression for the order parameter squared, namely S2 = r(eff)o/rTo, where rTo is the vitrified steady-state excitation anisotropy, we recovered an S2 of 0.75 for W59 fluorescence in uncomplexed FKBP12 and S2 approximately equal to 1 in the FKBP12/FK506 complex. Results obtained for the FKBP12/rapamycin complex are similar to those found for the FKBP12/FK506 complex. Minimum perturbation mapping simulations were performed on the free and complexed forms of FKBP12 and the results were generally in agreement with the experimental data.
机译:FK506结合蛋白(FKBP12)在FK506和雷帕霉素的免疫抑制作用中很重要。我们通过测量Trp时间分辨的荧光各向异性衰减r(t),研究了有或没有结合免疫抑制剂的FKBP12中的Trp侧链动力学。用单指数很好地描述了在20°C的水溶液中非复合FKBP12中W59的r(t),回收的初始各向异性r(eff)o为0.192,蛋白质的总旋转相关时间phi p为。 4.7 ns;对于FKBP12 / FK506复合体,r(eff)o = 0.214和phi p = 4.2 ns。使用顺序参数平方的表达式,即S2 = r(eff)o / rTo,其中rTo是玻璃化的稳态激发各向异性,我们获得了W59荧光在未复杂的FKBP12中的S2为0.75,而S2大约等于1。 FKBP12 / FK506复合体。 FKBP12 /雷帕霉素复合物获得的结果与FKBP12 / FK506复合物获得的结果相似。在自由和复杂形式的FKBP12上进行了最小扰动映射模拟,结果通常与实验数据一致。

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