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    Experiments in Nanomechanical Properties of Live Osteoblast Cells and Cell–Biomaterial Interface

    Source: Journal of Nanotechnology in Engineering and Medicine:;2011:;volume( 002 ):;issue: 004::page 41005
    Author:
    Rohit Khanna
    ,
    Kalpana S. Katti
    ,
    Dinesh R. Katti
    DOI: 10.1115/1.4005666
    Publisher: The American Society of Mechanical Engineers (ASME)
    Abstract: Characterizing the mechanical characteristics of living cells and cell–biomaterial composite is an important area of research in bone tissue engineering. In this work, an in situ displacement-controlled nanoindentation technique (using Hysitron Triboscope) is developed to perform nanomechanical characterization of living cells (human osteoblasts) and cell–substrate constructs under physiological conditions (cell culture medium; 37 °C). In situ elastic moduli (E) of adsorbed proteins on tissue culture polystyrene (TCPS) under cell culture media were found to be ∼4 GPa as revealed by modulus mapping experiments. The TCPS substrates soaked in cell culture medium showed significant difference in surface nanomechanical properties (up to depths of ∼12 nm) as compared to properties obtained from deeper indentations. Atomic force microscopy (AFM) revealed the cytoskeleton structures such as actin stress fiber networks on flat cells which are believed to impart the structural integrity to cell structure. Load-deformation response of cell was found to be purely elastic in nature, i.e., cell recovers its shape on unloading as indicated by linear loading and unloading curves obtained at 1000 nm indentation depth. The elastic response of cells is obtained during initial cell adhesion (ECell, 1 h, 1000 nm = 4.4–12.4 MPa), cell division (ECell, 2 days, 1000 nm = 1.3–3.0 MPa), and cell spreading (ECell, 2 days, 1000 nm = 6.9–11.6 MPa). Composite nanomechanical responses of cell–TCPS constructs were obtained by indentation at depths of 2000 nm and 3000 nm on cell-seeded TCPS. Elastic properties of cell–substrate composites were mostly dominated by stiff TCPS (EBulk = 5 GPa) lying underneath the cell.
    keyword(s): Deformation , Atomic force microscopy , Biomaterials , Stress , Mechanical properties , Displacement , Elastic moduli , Nanoindentation , Shapes , Physiology , Osteoblasts , Composite materials , Biological cells , Elasticity , Fluids , Fibers , Biological tissues , Proteins , Bone , Force AND Cultured cells ,
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      Experiments in Nanomechanical Properties of Live Osteoblast Cells and Cell–Biomaterial Interface

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    http://yetl.yabesh.ir/yetl1/handle/yetl/147287
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    contributor authorRohit Khanna
    contributor authorKalpana S. Katti
    contributor authorDinesh R. Katti
    date accessioned2017-05-09T00:46:15Z
    date available2017-05-09T00:46:15Z
    date copyrightNovember, 2011
    date issued2011
    identifier issn1949-2944
    identifier otherJNEMAA-28072#041005_1.pdf
    identifier urihttp://yetl.yabesh.ir/yetl/handle/yetl/147287
    description abstractCharacterizing the mechanical characteristics of living cells and cell–biomaterial composite is an important area of research in bone tissue engineering. In this work, an in situ displacement-controlled nanoindentation technique (using Hysitron Triboscope) is developed to perform nanomechanical characterization of living cells (human osteoblasts) and cell–substrate constructs under physiological conditions (cell culture medium; 37 °C). In situ elastic moduli (E) of adsorbed proteins on tissue culture polystyrene (TCPS) under cell culture media were found to be ∼4 GPa as revealed by modulus mapping experiments. The TCPS substrates soaked in cell culture medium showed significant difference in surface nanomechanical properties (up to depths of ∼12 nm) as compared to properties obtained from deeper indentations. Atomic force microscopy (AFM) revealed the cytoskeleton structures such as actin stress fiber networks on flat cells which are believed to impart the structural integrity to cell structure. Load-deformation response of cell was found to be purely elastic in nature, i.e., cell recovers its shape on unloading as indicated by linear loading and unloading curves obtained at 1000 nm indentation depth. The elastic response of cells is obtained during initial cell adhesion (ECell, 1 h, 1000 nm = 4.4–12.4 MPa), cell division (ECell, 2 days, 1000 nm = 1.3–3.0 MPa), and cell spreading (ECell, 2 days, 1000 nm = 6.9–11.6 MPa). Composite nanomechanical responses of cell–TCPS constructs were obtained by indentation at depths of 2000 nm and 3000 nm on cell-seeded TCPS. Elastic properties of cell–substrate composites were mostly dominated by stiff TCPS (EBulk = 5 GPa) lying underneath the cell.
    publisherThe American Society of Mechanical Engineers (ASME)
    titleExperiments in Nanomechanical Properties of Live Osteoblast Cells and Cell–Biomaterial Interface
    typeJournal Paper
    journal volume2
    journal issue4
    journal titleJournal of Nanotechnology in Engineering and Medicine
    identifier doi10.1115/1.4005666
    journal fristpage41005
    identifier eissn1949-2952
    keywordsDeformation
    keywordsAtomic force microscopy
    keywordsBiomaterials
    keywordsStress
    keywordsMechanical properties
    keywordsDisplacement
    keywordsElastic moduli
    keywordsNanoindentation
    keywordsShapes
    keywordsPhysiology
    keywordsOsteoblasts
    keywordsComposite materials
    keywordsBiological cells
    keywordsElasticity
    keywordsFluids
    keywordsFibers
    keywordsBiological tissues
    keywordsProteins
    keywordsBone
    keywordsForce AND Cultured cells
    treeJournal of Nanotechnology in Engineering and Medicine:;2011:;volume( 002 ):;issue: 004
    contenttypeFulltext
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