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首页> 外文期刊>Journal of cell biology >A novel split kinesin assay identifies motor proteins that interact with distinct vesicle populations
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A novel split kinesin assay identifies motor proteins that interact with distinct vesicle populations

机译:一种新颖的分裂驱动蛋白测定法可识别与不同囊泡群体相互作用的运动蛋白

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Identifying the kinesin motors that interact with different vesicle populations is a longstanding and challenging problem with implications for many aspects of cell biology. Here we introduce a new live-cell assay to assess kinesin–vesicle interactions and use it to identify kinesins that bind to vesicles undergoing dendrite-selective transport in cultured hippocampal neurons. We prepared a library of “split kinesins,” comprising an axon-selective kinesin motor domain and a series of kinesin tail domains that can attach to their native vesicles; when the split kinesins were assembled by chemical dimerization, bound vesicles were misdirected into the axon. This method provided highly specific results, showing that three Kinesin-3 family members—KIF1A, KIF13A, and KIF13B—interacted with dendritic vesicle populations. This experimental paradigm allows a systematic approach to evaluate motor–vesicle interactions in living cells.
机译:识别与不同囊泡群体相互作用的驱动蛋白运动是一个长期存在的挑战性问题,对细胞生物学的许多方面都有影响。在这里,我们介绍了一种新的活细胞测定法,以评估驱动蛋白与囊泡的相互作用,并用于鉴定与在培养的海马神经元中经历树突选择性转运的囊泡结合的驱动蛋白。我们准备了一个“分裂驱动蛋白”库,其中包括轴突选择性驱动蛋白运动域和一系列可连接至其天然囊泡的驱动蛋白尾部域。当分裂的驱动蛋白通过化学二聚化组装时,结合的囊泡被错误地定向到轴突中。该方法提供了高度特异性的结果,表明三个Kinesin-3家族成员KIF1A,KIF13A和KIF13B与树突状囊泡群体相互作用。这种实验范式允许系统地评估活细胞中的运动-囊泡相互作用。

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