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定量研究网格蛋白包被小窝与货物分子之间的动态相互作用。

Quantifying the dynamic interactions between a clathrin-coated pit and cargo molecules.

机构信息

School of Biomedical Engineering and Departments of Biomedical Sciences, Biochemistry and Molecular Biology, and Electrical and Computer Engineering, Colorado State University, Fort Collins, CO 80523.

出版信息

Proc Natl Acad Sci U S A. 2013 Nov 26;110(48):E4591-600. doi: 10.1073/pnas.1315202110. Epub 2013 Nov 11.

Abstract

Clathrin-mediated endocytosis takes place through the recruitment of cargo molecules into a growing clathrin-coated pit (CCP). Despite the importance of this process to all mammalian cells, little is yet known about the interaction dynamics between cargo and CCPs. These interactions are difficult to study because CCPs display a large degree of lifetime heterogeneity and the interactions with cargo molecules are time dependent. We use single-molecule total internal reflection fluorescence microscopy, in combination with automatic detection and tracking algorithms, to directly visualize the recruitment of individual voltage-gated potassium channels into forming CCPs in living cells. We observe association and dissociation of individual channels with a CCP and, occasionally, their internalization. Contrary to widespread ideas, cargo often escapes from a pit before abortive CCP termination or endocytic vesicle production. Thus, the binding times of cargo molecules associating to CCPs are much shorter than the overall endocytic process. By measuring tens of thousands of capturing events, we build the distribution of capture times and the times that cargo remains confined to a CCP. An analytical stochastic model is developed and compared with the measured distributions. Due to the dynamic nature of the pit, the model is non-Markovian and it displays long-tail power law statistics. The measured distributions and model predictions are in excellent agreement over more than five orders of magnitude. Our findings identify one source of the large heterogeneities in CCP dynamics and provide a mechanism for the anomalous diffusion of proteins in the plasma membrane.

摘要

网格蛋白介导的内吞作用是通过将货物分子募集到不断生长的网格蛋白包被陷窝(CCP)中进行的。尽管这个过程对所有哺乳动物细胞都很重要,但我们对货物与 CCP 之间的相互作用动力学还知之甚少。这些相互作用很难研究,因为 CCP 显示出很大程度的寿命异质性,并且与货物分子的相互作用是时间依赖性的。我们使用单分子全内反射荧光显微镜,结合自动检测和跟踪算法,直接观察电压门控钾通道在活细胞中形成 CCP 时的单个通道募集情况。我们观察到单个通道与 CCP 的结合和解离,偶尔还观察到它们的内化。与普遍的观点相反,货物分子在无效的 CCP 终止或内吞小泡产生之前常常从陷窝中逃逸。因此,货物分子与 CCP 结合的结合时间比整个内吞过程短得多。通过测量数万次捕获事件,我们构建了捕获时间和货物分子限制在 CCP 中的时间的分布。开发了一个分析随机模型,并将其与测量的分布进行比较。由于陷窝的动态性质,该模型是非马尔可夫的,并且显示出长尾幂律统计。在五个数量级以上的范围内,测量的分布和模型预测非常吻合。我们的发现确定了 CCP 动力学中大量异质性的一个来源,并为蛋白质在质膜中的异常扩散提供了一种机制。

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