Literature DB >> 21468318

Three-dimensional traction force microscopy: a new tool for quantifying cell-matrix interactions.

Christian Franck1, Stacey A Maskarinec, David A Tirrell, Guruswami Ravichandran.   

Abstract

The interactions between biochemical processes and mechanical signaling play important roles during various cellular processes such as wound healing, embryogenesis, metastasis, and cell migration. While tn class="Gene">raditional traction force measurements have provided quantitative information about cell matrix interactions in two dimensions, recent studies have shown significant differences in the behavior and morphology of cells when placed in three-dimensional environments. Hence new quantitative experimental techniques are needed to accurately determine cell traction forces in three dimensions. Recently, two approaches both based on laser scanning confocal microscopy have emerged to address this need. This study highlights the details, implementation and advantages of such a three-dimensional imaging methodology with the capability to compute cellular traction forces dynamically during cell migration and locomotion. An application of this newly developed three-dimensional traction force microscopy (3D TFM) technique to single cell migration studies of 3T3 fibroblasts is presented to show that this methodology offers a new quantitative vantage point to investigate the three-dimensional nature of cell-ECM interactions.

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Year:  2011        PMID: 21468318      PMCID: PMC3066163          DOI: 10.1371/journal.pone.0017833

Source DB:  PubMed          Journal:  PLoS One        ISSN: 1932-6203            Impact factor:   3.240


  34 in total

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6.  Traction forces in locomoting cells.

Authors:  T Oliver; M Dembo; K Jacobson
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  82 in total

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Review 6.  Role of the extracellular matrix in regulating stem cell fate.

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Review 7.  Toward single cell traction microscopy within 3D collagen matrices.

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10.  Fiber based optical tweezers for simultaneous in situ force exertion and measurements in a 3D polyacrylamide gel compartment.

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