Literature DB >> 20473350

Neutrophil adhesion and chemotaxis depend on substrate mechanics.

Risat A Jannat1, Gregory P Robbins, Brendon G Ricart, Micah Dembo, Daniel A Hammer.   

Abstract

Neutrophil adhesion to the vasculature and chemotaxis within tissues play critical roles in the inflammatory response to injury and pathogens. Unregulated neutrophil activity has been implicated in the progression of numerous chronic and acute diseases such as rheumatoid arthritis, asthma, and sepsis. Cell migration of anchorage-dependent cells is known to depend on both chemical and mechanical interactions. Although neutrophil responses to chemical cues have been well characterized, little is known about the effect of underlying tissue mechanics on neutrophil adhesion and migration. To address this question, we quantified neutrophil migration and traction stresses on compliant hydrogel substrates with varying elasticity in a micro-machined gradient chamber in which we could apply either a uniform concentration or a precise gradient of the bacterial chemoattractant fMLP. Neutrophils spread more extensively on substrates of greater stiffness. In addition, increasing the stiffness of the substrate leads to a significant increase in the chemotactic index for each fMLP gradient tested. As the substrate becomes stiffer, neutrophils generate higher traction forces without significant changes in cell speed. These forces are often displayed in pairs and focused in the uropod. Increases in the mean fMLP concentration beyond the K(D) of the receptor lead to a decrease in chemotactic index on all surfaces. Blocking with an antibody against beta(2)-integrins leads to a significant reduction but not an elimination of directed motility on stiff materials, but no change in motility on soft materials, suggesting neutrophils can display both integrin-dependent and integrin-independent motility. These findings are critical for understanding how neutrophil migration may change in different mechanical environments in vivo and can be used to guide the design of migration inhibitors that more efficiently target inflammation.

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Year:  2010        PMID: 20473350      PMCID: PMC2867619          DOI: 10.1088/0953-8984/22/19/194117

Source DB:  PubMed          Journal:  J Phys Condens Matter        ISSN: 0953-8984            Impact factor:   2.333


  40 in total

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3.  Neutrophil traction stresses are concentrated in the uropod during migration.

Authors:  Lee A Smith; Helim Aranda-Espinoza; Jered B Haun; Micah Dembo; Daniel A Hammer
Journal:  Biophys J       Date:  2007-01-11       Impact factor: 4.033

Review 4.  Substrate rigidity and force define form through tyrosine phosphatase and kinase pathways.

Authors:  Grégory Giannone; Michael P Sheetz
Journal:  Trends Cell Biol       Date:  2006-03-10       Impact factor: 20.808

5.  Neutrophil morphology and migration are affected by substrate elasticity.

Authors:  Patrick W Oakes; Dipan C Patel; Nicole A Morin; Daniel P Zitterbart; Ben Fabry; Jonathan S Reichner; Jay X Tang
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Review 6.  Cells on the run: shear-regulated integrin activation in leukocyte rolling and arrest on endothelial cells.

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  36 in total

1.  Measuring traction forces of motile dendritic cells on micropost arrays.

Authors:  Brendon G Ricart; Michael T Yang; Christopher A Hunter; Christopher S Chen; Daniel A Hammer
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2.  Protrusive and Contractile Forces of Spreading Human Neutrophils.

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3.  Controlling the mechanical properties of three-dimensional matrices via non-enzymatic collagen glycation.

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4.  Finite element analysis of traction force microscopy: influence of cell mechanics, adhesion, and morphology.

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Review 5.  Toward single cell traction microscopy within 3D collagen matrices.

Authors:  Matthew S Hall; Rong Long; Xinzeng Feng; Yuling Huang; Chung-Yuen Hui; Mingming Wu
Journal:  Exp Cell Res       Date:  2013-06-25       Impact factor: 3.905

6.  Traction forces of neutrophils migrating on compliant substrates.

Authors:  Risat A Jannat; Micah Dembo; Daniel A Hammer
Journal:  Biophys J       Date:  2011-08-03       Impact factor: 4.033

7.  Endothelial cell substrate stiffness influences neutrophil transmigration via myosin light chain kinase-dependent cell contraction.

Authors:  Kimberly M Stroka; Helim Aranda-Espinoza
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8.  The RhoA guanine nucleotide exchange factor, LARG, mediates ICAM-1-dependent mechanotransduction in endothelial cells to stimulate transendothelial migration.

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9.  Macrophage motility is driven by frontal-towing with a force magnitude dependent on substrate stiffness.

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