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    Date Issued2015 (2)AuthorGrunwald, David (2)
    Joseph, Aviva (2)
    Smith, Carlas (2)Abrahamsson, Sara (1)Dange, Thomas (1)View MoreUMass Chan AffiliationRNA Therapeutics Institute (2)Department Biochemistry and Molecular Pharmacology (1)Document TypeJournal Article (2)KeywordCell Biology (2)Actins (1)Animals (1)Biochemistry, Biophysics, and Structural Biology (1)Cell and Developmental Biology (1)View MoreJournalThe Journal of cell biology (2)

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    In vivo single-particle imaging of nuclear mRNA export in budding yeast demonstrates an essential role for Mex67p

    Smith, Carlas; Lari, Azra; Derrer, Carina Patrizia.; Ouwehand, Anette; Rossouw, Ammeret; Huisman, Maximiliaan; Dange, Thomas; Hopman, Mark; Joseph, Aviva; Zenklusen, Daniel; et al. (2015-12-21)
    Many messenger RNA export proteins have been identified; yet the spatial and temporal activities of these proteins and how they determine directionality of messenger ribonucleoprotein (mRNP) complex export from the nucleus remain largely undefined. Here, the bacteriophage PP7 RNA-labeling system was used in Saccharomyces cerevisiae to follow single-particle mRNP export events with high spatial precision and temporal resolution. These data reveal that mRNP export, consisting of nuclear docking, transport, and cytoplasmic release from a nuclear pore complex (NPC), is fast ( approximately 200 ms) and that upon arrival in the cytoplasm, mRNPs are frequently confined near the nuclear envelope. Mex67p functions as the principal mRNP export receptor in budding yeast. In a mex67-5 mutant, delayed cytoplasmic release from NPCs and retrograde transport of mRNPs was observed. This proves an essential role for Mex67p in cytoplasmic mRNP release and directionality of transport.
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    Nuclear accessibility of beta-actin mRNA is measured by 3D single-molecule real-time tracking

    Smith, Carlas; Preibisch, Stephan; Joseph, Aviva; Abrahamsson, Sara; Rieger, Bernd; Myers, Eugene; Singer, Robert H.; Grunwald, David (2015-05-25)
    Imaging single proteins or RNAs allows direct visualization of the inner workings of the cell. Typically, three-dimensional (3D) images are acquired by sequentially capturing a series of 2D sections. The time required to step through the sample often impedes imaging of large numbers of rapidly moving molecules. Here we applied multifocus microscopy (MFM) to instantaneously capture 3D single-molecule real-time images in live cells, visualizing cell nuclei at 10 volumes per second. We developed image analysis techniques to analyze messenger RNA (mRNA) diffusion in the entire volume of the nucleus. Combining MFM with precise registration between fluorescently labeled mRNA, nuclear pore complexes, and chromatin, we obtained globally optimal image alignment within 80-nm precision using transformation models. We show that beta-actin mRNAs freely access the entire nucleus and fewer than 60% of mRNAs are more than 0.5 microm away from a nuclear pore, and we do so for the first time accounting for spatial inhomogeneity of nuclear organization.
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