PKCδ localization at the membrane increases matrix traction force dependent on PLCγ1/EGFR signaling.

PKCδ localization at the membrane increases matrix traction force dependent on PLCγ1/EGFR signaling.

INTRODUCTION:During wound healing, fibroblasts initially migrate into the wound bed and later contract the matrix. Relevant mediators of transcellular contractility revealed by systems analyses are protein kinase c delta/myosin light chain-2 (PKCδ/MLC-2). PKCδ is activated by growth factor-driven PL...

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Main Authors: Joshua Jamison, Douglas Lauffenburger, James C-H Wang, Alan Wells
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2013-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC3796482?pdf=render
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spelling doaj-6f47c3e0dcd943f6acf0ee63d3aeabd72020-11-25T01:19:26ZengPublic Library of Science (PLoS)PLoS ONE1932-62032013-01-01810e7743410.1371/journal.pone.0077434PKCδ localization at the membrane increases matrix traction force dependent on PLCγ1/EGFR signaling.Joshua JamisonDouglas LauffenburgerJames C-H WangAlan WellsINTRODUCTION:During wound healing, fibroblasts initially migrate into the wound bed and later contract the matrix. Relevant mediators of transcellular contractility revealed by systems analyses are protein kinase c delta/myosin light chain-2 (PKCδ/MLC-2). PKCδ is activated by growth factor-driven PLCγ1 hydrolysis of phosphoinositide bisphosphate (PIP2) hydrolysis when it becomes tranlocated to the membrane. This leads to MLC-2 phosphorylation that regulates myosin for contractility. Furthermore, PKCδ n-terminus mediates PKCδ localization to the membrane in relative proximity to PLCγ1 activity. However, the role this localization and the relationship to its activation and signaling of force is not well understood. Therefore, we investigated whether the membrane localization of PKCδ mediates the transcellular contractility of fibroblasts. METHODS:To determine PKCδ activation in targeted membrane locations in mouse fibroblast cells (NR6-WT), two PKCδ constructs were generated; PKCδ-CaaX with farnesylation moiety targeting PKCδ to the membrane and PKCδ-SaaX a non-targeting control. RESULTS:Increased mean cell force was observed before and during EGF stimulation in fibroblasts expressing membrane-targeted PKCδ (PKCδ-CaaX) when analyzed with 2D cell traction force and 3D compaction of collagen matrix. This effect was reduced in cells deficient in EGFR/PLCy1 signaling. In cells expressing non-membrane targeted PKCδ (PKCδ-SaaX), the cell force exerted outside the ECM (extracellular matrix) was less, but cell motility/speed/persistence was increased after EGF stimulation. Change in cell motility and increased force exertion was also preceded by change in cell morphology. Organization of actin stress fibers was also decreased as a result of increasing membrane targeting of PKCδ. CONCLUSION:From these results membrane tethering of PKCδ leads to increased force exertion on ECM. Furthermore, our data show PLCγ1 regulation of PKCδ, at least in part, drives transcellular contractility in fibroblasts.http://europepmc.org/articles/PMC3796482?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Joshua Jamison
Douglas Lauffenburger
James C-H Wang
Alan Wells
spellingShingle Joshua Jamison
Douglas Lauffenburger
James C-H Wang
Alan Wells
PKCδ localization at the membrane increases matrix traction force dependent on PLCγ1/EGFR signaling.
PLoS ONE
author_facet Joshua Jamison
Douglas Lauffenburger
James C-H Wang
Alan Wells
author_sort Joshua Jamison
title PKCδ localization at the membrane increases matrix traction force dependent on PLCγ1/EGFR signaling.
title_short PKCδ localization at the membrane increases matrix traction force dependent on PLCγ1/EGFR signaling.
title_full PKCδ localization at the membrane increases matrix traction force dependent on PLCγ1/EGFR signaling.
title_fullStr PKCδ localization at the membrane increases matrix traction force dependent on PLCγ1/EGFR signaling.
title_full_unstemmed PKCδ localization at the membrane increases matrix traction force dependent on PLCγ1/EGFR signaling.
title_sort pkcδ localization at the membrane increases matrix traction force dependent on plcγ1/egfr signaling.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2013-01-01
description INTRODUCTION:During wound healing, fibroblasts initially migrate into the wound bed and later contract the matrix. Relevant mediators of transcellular contractility revealed by systems analyses are protein kinase c delta/myosin light chain-2 (PKCδ/MLC-2). PKCδ is activated by growth factor-driven PLCγ1 hydrolysis of phosphoinositide bisphosphate (PIP2) hydrolysis when it becomes tranlocated to the membrane. This leads to MLC-2 phosphorylation that regulates myosin for contractility. Furthermore, PKCδ n-terminus mediates PKCδ localization to the membrane in relative proximity to PLCγ1 activity. However, the role this localization and the relationship to its activation and signaling of force is not well understood. Therefore, we investigated whether the membrane localization of PKCδ mediates the transcellular contractility of fibroblasts. METHODS:To determine PKCδ activation in targeted membrane locations in mouse fibroblast cells (NR6-WT), two PKCδ constructs were generated; PKCδ-CaaX with farnesylation moiety targeting PKCδ to the membrane and PKCδ-SaaX a non-targeting control. RESULTS:Increased mean cell force was observed before and during EGF stimulation in fibroblasts expressing membrane-targeted PKCδ (PKCδ-CaaX) when analyzed with 2D cell traction force and 3D compaction of collagen matrix. This effect was reduced in cells deficient in EGFR/PLCy1 signaling. In cells expressing non-membrane targeted PKCδ (PKCδ-SaaX), the cell force exerted outside the ECM (extracellular matrix) was less, but cell motility/speed/persistence was increased after EGF stimulation. Change in cell motility and increased force exertion was also preceded by change in cell morphology. Organization of actin stress fibers was also decreased as a result of increasing membrane targeting of PKCδ. CONCLUSION:From these results membrane tethering of PKCδ leads to increased force exertion on ECM. Furthermore, our data show PLCγ1 regulation of PKCδ, at least in part, drives transcellular contractility in fibroblasts.
url http://europepmc.org/articles/PMC3796482?pdf=render
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