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    Investigation of Cellular Confinement in Three-Dimensional Microscale Fibrous Substrates: Fabrication and Metrology

    Source: Journal of Micro and Nano-Manufacturing:;2018:;volume( 006 ):;issue: 002::page 21003
    Author:
    Tourlomousis, Filippos
    ,
    Boettcher, William
    ,
    Ding, Houzhu
    ,
    Chang, Robert C.
    DOI: 10.1115/1.4038803
    Publisher: The American Society of Mechanical Engineers (ASME)
    Abstract: Engineered microenvironments along with robust quantitative models of cell shape metrology that can decouple the effect of various well-defined cues on a stem cell's phenotypic response would serve as an illuminating tool for testing mechanistic hypotheses on how stem cell fate is fundamentally regulated. As an experimental testbed to probe the effect of geometrical confinement on cell morphology, three-dimensional (3D) poly(ε-caprolactone) (PCL) layered fibrous meshes are fabricated with an in-house melt electrospinning writing system (MEW). Gradual confinement states of fibroblasts are demonstrated by seeding primary fibroblasts on defined substrates, including a classical two-dimensional (2D) petri dish and porous 3D fibrous substrates with microarchitectures tunable within a tight cellular dimensional scale window (1–50 μm). To characterize fibroblast confinement, a quantitative 3D confocal fluorescence imaging workflow for 3D cell shape representation is presented. The methodology advanced allows the extraction of cellular and subcellular morphometric features including the number, location, and 3D distance distribution metrics of the shape-bearing focal adhesion (FA) proteins.
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      Investigation of Cellular Confinement in Three-Dimensional Microscale Fibrous Substrates: Fabrication and Metrology

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    contributor authorTourlomousis, Filippos
    contributor authorBoettcher, William
    contributor authorDing, Houzhu
    contributor authorChang, Robert C.
    date accessioned2019-02-28T11:05:13Z
    date available2019-02-28T11:05:13Z
    date copyright1/18/2018 12:00:00 AM
    date issued2018
    identifier issn2166-0468
    identifier otherjmnm_006_02_021003.pdf
    identifier urihttp://yetl.yabesh.ir/yetl1/handle/yetl/4252525
    description abstractEngineered microenvironments along with robust quantitative models of cell shape metrology that can decouple the effect of various well-defined cues on a stem cell's phenotypic response would serve as an illuminating tool for testing mechanistic hypotheses on how stem cell fate is fundamentally regulated. As an experimental testbed to probe the effect of geometrical confinement on cell morphology, three-dimensional (3D) poly(ε-caprolactone) (PCL) layered fibrous meshes are fabricated with an in-house melt electrospinning writing system (MEW). Gradual confinement states of fibroblasts are demonstrated by seeding primary fibroblasts on defined substrates, including a classical two-dimensional (2D) petri dish and porous 3D fibrous substrates with microarchitectures tunable within a tight cellular dimensional scale window (1–50 μm). To characterize fibroblast confinement, a quantitative 3D confocal fluorescence imaging workflow for 3D cell shape representation is presented. The methodology advanced allows the extraction of cellular and subcellular morphometric features including the number, location, and 3D distance distribution metrics of the shape-bearing focal adhesion (FA) proteins.
    publisherThe American Society of Mechanical Engineers (ASME)
    titleInvestigation of Cellular Confinement in Three-Dimensional Microscale Fibrous Substrates: Fabrication and Metrology
    typeJournal Paper
    journal volume6
    journal issue2
    journal titleJournal of Micro and Nano-Manufacturing
    identifier doi10.1115/1.4038803
    journal fristpage21003
    journal lastpage021003-7
    treeJournal of Micro and Nano-Manufacturing:;2018:;volume( 006 ):;issue: 002
    contenttypeFulltext
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    DSpace software copyright © 2002-2015  DuraSpace
    نرم افزار کتابخانه دیجیتال "دی اسپیس" فارسی شده توسط یابش برای کتابخانه های ایرانی | تماس با یابش
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