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Heterodimeric interaction and interfaces of S100A1 and S100P

机译:S100A1和S100P的异二聚体相互作用和界面

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摘要

With the widespread use of yeast two-hybrid systems, many heterodimeric forms of S100 proteins have been found, although their biological significance is unknown. In the present study, S100A1 was found to interact with another S100 protein, S100P, by using the yeast two-hybrid system. The binding parameters of the interaction were obtained using an optical biosensor and show that S100P has a slightly higher affinity for S100A1 (Kd=10–20 nM) when compared with that for self-association (Kd=40–120 nM). The physical interaction of S100A1 and S100P was also demonstrated in living mammalian cells using a fluorescence resonance energy transfer technique. Preincubation of recombinant S100P with S100A1, before the biosensor assay, reduced by up to 50% the binding of S100P to a recombinant C-terminal fragment of non-muscle myosin A, one of its target molecules. Site-specific mutations of S100P and S100A1, combined with homology modelling of an S100P/S100A1 heterodimer using known S100P and S100A1 structures, allowed the hydrophobic interactions at the dimeric interface of the heterodimer to be defined and provide an explanation for the heterodimerization of S100P and S100A1 at the molecular level. These results have revealed the similarities and the differences between the S100P homodimer and the S100A1/S100P heterodimer.
机译:随着酵母双杂交系统的广泛使用,已发现许多S100蛋白的异二聚体形式,尽管其生物学意义尚不清楚。在本研究中,通过使用酵母双杂交系统,发现S100A1与另一种S100蛋白S100P相互作用。相互作用的结合参数是使用光学生物传感器获得的,表明与自缔合(Kd = 40–120 nM)相比,S100P对S100A1的亲和力稍高(Kd = 10–20 nM)。还使用荧光共振能量转移技术在活的哺乳动物细胞中证明了S100A1和S100P的物理相互作用。在生物传感器测定之前,将重组S100P与S100A1预孵育,可使S100P与非肌肉肌球蛋白A(其靶分子之一)的重组C末端片段的结合降低多达50%。 S100P和S100A1的位点特异性突变,结合使用已知S100P和S100A1结构的S100P / S100A1异二聚体的同源性建模,可以定义异二聚体二聚体界面处的疏水相互作用,并为S100P和S100A的异二聚化提供解释S100A1在分子水平上。这些结果揭示了S100P同二聚体和S100A1 / S100P异二聚体之间的相似之处和不同之处。

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