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H-Ras Nanocluster Stability Regulates the Magnitude of MAPK Signal Output

机译:H-Ras纳米簇的稳定性调节MAPK信号输出的幅度

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摘要

H-Ras is a binary switch that is activated by multiple co-factors and triggers several key cellular pathways one of which is MAPK. The specificity and magnitude of downstream activation is achieved by the spatio-temporal organization of the active H-Ras in the plasma membrane. Upon activation, the GTP bound H-Ras binds to Galectin-1 (Gal-1) and becomes transiently immobilized in short-lived nanoclusters on the plasma membrane from which the signal is propagated to Raf. In the current study we show that stabilizing the H-Ras-Gal-1 interaction, using bimolecular fluorescence complementation (BiFC), leads to prolonged immobilization of H-Ras.GTP in the plasma membrane which was measured by fluorescence recovery after photobleaching (FRAP), and increased signal out-put to the MAPK module. EM measurements of Raf recruitment to the H-Ras.GTP nanoclusters demonstrated that the enhanced signaling observed in the BiFC stabilized H-Ras.GTP nanocluster was attributed to increased H-Ras immobilization rather than to an increase in Raf recruitment. Taken together these data demonstrate that the magnitude of the signal output from a GTP-bound H-Ras nanocluster is proportional to its stability.
机译:H-Ras是一个由多个辅助因子激活的二进制开关,可触发几种关键的细胞途径,其中之一是MAPK。下游激活的特异性和强度是通过质膜中活性H-Ras的时空组织来实现的。激活后,结合GTP的H-Ras与Galectin-1(Gal-1)结合,并暂时固定在质膜上的短寿命纳米团簇中,信号从该团簇传播至Raf。在当前的研究中,我们表明使用双分子荧光互补(BiFC)稳定H-Ras-Gal-1相互作用会导致H-Ras.GTP长时间固定在质膜上,这是通过光漂白后的荧光恢复(FRAP)来测量的),并增加了MAPK模块的信号输出。 EM测量Raf募集到H-Ras.GTP纳米簇表明,在BiFC稳定的H-Ras.GTP纳米簇中观察到的增强信号传导归因于H-Ras固定化的增加,而不是Raf募集的增加。这些数据加在一起表明从GTP结合的H-Ras纳米簇输出的信号的大小与其稳定性成正比。

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