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Formation of the Nuclear Envelope Permeability Barrier Studied by Sequential Photoswitching and Flux Analysis

机译:通过顺序光开关和通量分析研究核包膜渗透性屏障的形成

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摘要

In higher eukaryotes, the nuclear envelope breaks down during mitosis. It reforms during telophase, and nuclear import is reestablished within <10 min after anaphase onset. It is widely assumed that import functionality simultaneously leads to the exclusion of bulk cytoplasmic proteins. However, nuclear pore complex assembly is not fully completed when import capacity is regained, which raises the question of whether the transport and permeability barrier functions of the nuclear envelope are indeed coupled. In this study, we therefore analyzed the reestablishment of the permeability barrier of the nuclear envelope after mitosis in living cells by monitoring the flux of the reversibly photoswitchable fluorescent protein Dronpa from the cytoplasm into the nucleus after photoactivation. We performed many consecutive flux measurements in the same cell to directly monitor changes in nuclear envelope permeability. Our measurements at different time points after mitosis in individual cells show that contrary to the general view and despite the rapid reestablishment of facilitated nuclear import, the nuclear envelope remains relatively permeable for passive diffusion for the first 2 h after mitosis. Our data demonstrate that reformation of the permeability barrier of nuclear pore complexes occurs only gradually and is uncoupled from regaining active import functionality.
机译:在高等真核生物中,有核分裂过程中核被膜破裂。它在末期重新形成,并且在后期开始后不到10分钟内重新建立核输入。人们普遍认为,导入功能会同时导致大量胞质蛋白的排斥。然而,当重新获得进口能力时,核孔复合体的组装并未完全完成,这引发了核壳层的运输和渗透屏障功能是否确实耦合的问题。因此,在这项研究中,我们通过监测光激活后从细胞质到细胞核的可逆光开关荧光蛋白Dronpa的通量,分析了活细胞有丝分裂后核膜的通透性屏障的重建。我们在同一电池中执行了许多连续的通量测量,以直接监视核包膜通透性的变化。我们在单个细胞有丝分裂后不同时间点的测量结果表明,与一般观点相反,尽管快速重建了便利的核输入,但核包膜在有丝分裂后的前2小时内仍具有相对可渗透的被动扩散能力。我们的数据表明核孔复合物渗透屏障的重整仅是逐渐发生的,并且与重新获得主动进口功能无关。

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