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      The Effect of Cell Morphology on the Permeability of the Nuclear Envelope to Diffusive Factors

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          Abstract

          A recent advance in understanding stem cell differentiation is that the cell is able to translate its morphology, i.e., roundish or spread, into a fate decision. We hypothesize that strain states in the nuclear envelope (NE) cause changes in the structure of the nuclear pore complexes. This induces significant changes in the NE's permeability to the traffic of the transcription factors involved in stem cell differentiation which are imported into the nucleus by passive diffusion. To demonstrate this, we set up a numerical model of the transport of diffusive molecules through the nuclear pore complex (NPC), on the basis of the NPC deformation. We then compared the prediction of the model for two different cell configurations with roundish and spread nuclear topologies with those measured on cells cultured in both configurations. To measure the geometrical features of the NPC, using electron tomography we reconstructed three-dimensional portions of the envelope of cells cultured in both configurations. We found non-significant differences in both the shape and size of the transmembrane ring of single pores with envelope deformation. In the numerical model, we thus assumed that the changes in pore complex permeability, caused by the envelope strains, are due to variations in the opening configuration of the nuclear basket, which in turn modifies the porosity of the pore complex mainly on its nuclear side. To validate the model, we cultured cells on a substrate shaped as a spatial micro-grid, called the “nichoid,” which is nanoengineered by two-photon laser polymerization, and induces a roundish nuclear configuration in cells adhering to the nichoid grid, and a spread configuration in cells adhering to the flat substrate surrounding the grid. We then measured the diffusion through the nuclear envelope of an inert green-fluorescent protein, by fluorescence recovery after photobleaching (FRAP). Finally, we compared the diffusion times predicted by the numerical model for roundish vs. spread cells, with the measured times. Our data show that cell stretching modulates the characteristic time needed for the nuclear import of a small inert molecule, GFP, and the model predicts a faster import of diffusive molecules in the spread compared to roundish cells.

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          The green fluorescent protein.

          R Tsien (1998)
          In just three years, the green fluorescent protein (GFP) from the jellyfish Aequorea victoria has vaulted from obscurity to become one of the most widely studied and exploited proteins in biochemistry and cell biology. Its amazing ability to generate a highly visible, efficiently emitting internal fluorophore is both intrinsically fascinating and tremendously valuable. High-resolution crystal structures of GFP offer unprecedented opportunities to understand and manipulate the relation between protein structure and spectroscopic function. GFP has become well established as a marker of gene expression and protein targeting in intact cells and organisms. Mutagenesis and engineering of GFP into chimeric proteins are opening new vistas in physiological indicators, biosensors, and photochemical memories.
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            Green fluorescent protein as a marker for gene expression.

            Keith W. Ward, D Prasher, M Chalfie (1994)
            A complementary DNA for the Aequorea victoria green fluorescent protein (GFP) produces a fluorescent product when expressed in prokaryotic (Escherichia coli) or eukaryotic (Caenorhabditis elegans) cells. Because exogenous substrates and cofactors are not required for this fluorescence, GFP expression can be used to monitor gene expression and protein localization in living organisms.
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              Studying protein dynamics in living cells.

              J. Lippincott-Schwartz, E Snapp, A Kenworthy (2001)
              Since the advent of the green fluorescent protein, the subcellular localization, mobility, transport routes and binding interactions of proteins can be studied in living cells. Live cell imaging, in combination with photobleaching, energy transfer or fluorescence correlation spectroscopy are providing unprecedented insights into the movement of proteins and their interactions with cellular components. Remarkably, these powerful techniques are accessible to non-specialists using commercially available microscope systems.
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                Author and article information

                Contributors
                Journal
                Journal ID (nlm-ta): Front Physiol
                Journal ID (iso-abbrev): Front Physiol
                Journal ID (publisher-id): Front. Physiol.
                Title: Frontiers in Physiology
                Publisher: Frontiers Media S.A.
                ISSN (Electronic): 1664-042X
                Publication date (Electronic): 13 July 2018
                Publication date Collection: 2018
                Volume: 9
                Electronic Location Identifier: 925
                Affiliations
                [1] 1Laboratori de Càlcul Numèric, E.T.S. de Ingenieros de Caminos, Canales y Puertos, Universitat Politècnica de Catalunya – (UPC BarcelonaTech) , Barcelona, Spain
                [2] 2Department of Chemistry, Materials and Chemical Engineeering “Giulio Natta, ” Politecnico di Milano , Milan, Italy
                [3] 3Electron Microscopy Facility, Istituto Italiano di Tecnologia , Genoa, Italy
                [4] 4Unità di Ricerca Consorzio INSTM, Politecnico di Milano , Milan, Italy
                Author notes

                Edited by: Mariano Vázquez, Barcelona Supercomputing Center, Spain

                Reviewed by: Chiara Giverso, Politecnico di Torino, Italy; Hermann Frieboes, University of Louisville, United States

                *Correspondence: Alberto García-González berto.garcia@ 123456upc.edu

                This article was submitted to Computational Physiology and Medicine, a section of the journal Frontiers in Physiology

                †These authors have contributed equally to this work.

                Article
                DOI: 10.3389/fphys.2018.00925
                PMC ID: 6053530
                PubMed ID: 30057558
                SO-VID: aa120fa7-5add-41e8-8343-bc67cede2447
                Copyright © Copyright © 2018 García-González, Jacchetti, Marotta, Tunesi, Rodríguez Matas and Raimondi.
                License:

                This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) and the copyright owner(s) are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.

                History
                Date received : 30 March 2018
                Date accepted : 25 June 2018
                Page count
                Figures: 10, Tables: 2, Equations: 13, References: 42, Pages: 15, Words: 10351
                Funding
                Funded by: H2020 European Research Council 10.13039/100010663
                Award ID: grant agreement No. 646990 - NICHOID
                Categories
                Subject: Physiology
                Subject: Original Research

                ScienceOpen disciplines: Anatomy & Physiology
                Keywords: nuclear pore complex,passive diffusion,nuclear envelope permeability,stem cell differentiation,finite element modeling,scanning transmission electron microscopy,confocal microscopy
                Data availability:
                ScienceOpen disciplines: Anatomy & Physiology
                Keywords: nuclear pore complex, passive diffusion, nuclear envelope permeability, stem cell differentiation, finite element modeling, scanning transmission electron microscopy, confocal microscopy

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