Epithelial monolayer wounding stimulates binding of USF-1 to an E-box motif in the plasminogen activator inhibitor type 1 gene

doi:10.1242/jcs.00051

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doi: 10.1242/10.1242/jcs.00051

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Journal of Cell Science 115, 3767-3777 (2002)
Copyright © 2002 The Company of Biologists Limited
doi: 10.1242/jcs.00051

Research Article

Epithelial monolayer wounding stimulates binding of USF-1 to an E-box motif in the plasminogen activator inhibitor type 1 gene

Kirwin M. Providence¹, Lisa A. White¹, Jianzhong Tang¹, John Gonclaves², Lisa Staiano-Coico² and Paul J. Higgins¹^,*

^¹ Center for Cell Biology & Cancer Research, Albany Medical College, Albany, NY 12208, USA
^² Department of Surgery, Weill Medical College of Cornell University, New York, NY 10021, USA

^* Author for correspondence (e-mail: higginp{at}mail.amc.edu)

Accepted 9 July 2002

Several proteases and their co-expressed inhibitors modulatethe interdependent processes of cell migration and matrix proteolysisduring wound repair. Transcription of the gene encoding plasminogenactivator inhibitor type 1 (PAI-1), a serine protease inhibitorimportant in the control of barrier proteolysis and cell-to-matrixadhesion, is spatially-temporally regulated following epithelialdenudation injury in vitro as well as in vivo. Using a well-definedculture model of acute epidermal wounding and reepithelialization,PAI-1 mRNA/protein synthesis was induced early after monolayerscraping and restricted to cells comprising the motile cohort.PAI-1 levels in locomoting cells remained elevated (relativeto the distal, contact-inhibited monolayer regions) throughoutthe time course of trauma repair. Targeted PAI-1 downregulationby transfection of antisense PAI-1 expression constructs significantlyimpaired keratinocyte migration and monolayer scrape wound closure.Injury-induced PAI-1 transcription closely paralleled growthstate-dependent controls on the PAI-1 gene. An E-box motif (CACGTG)in the PAI-1 proximal promoter (located at nucleotides -160to -165), previously shown to be necessary for serum-inducedPAI-1 expression, was bound by nuclear factors from wound-stimulatedbut not quiescent, contact-inhibited, keratinocytes. UV crosslinkingapproaches to identify E-box-binding factors coupled with deoxyoligonucleotideaffinity chromatography and gel retardation assays confirmedat least one major E-box-binding protein in both serum- and wound-activatedcells to be USF-1, a member of the helix-loop-helix family of transcriptionfactors. An intact hexanucleotide E-box motif was necessaryand sufficient for USF-1 binding using nuclear extracts fromboth serum- and wound-simulated cells. Two species of immunoreactiveUSF-1 were identified by western blotting of total cellularlysates that corresponded to the previously characterized phosphorylatedand non-phosphorylated forms of the protein. USF-1 isolatedby PAI-1 promoter-DNA affinity chromatography was almost exclusivelyphosphorylated. Only a fraction of the total cellular USF-1in proliferating cultures, by comparison, was phosphorylatedat any given time. PAI-1 E-box binding activity, assessed byprobe mobility shift criteria, increased within 2 hours of monolayerscrape injury, a time frame consistent with wound-stimulatedincreases in PAI-1 transcription. Relative to intact cultures,scrape site-juxtaposed cells had significantly greater cytoplasmic andnuclear USF-1 immunoreactivity correlating with the specificin situ-restricted expression of PAI-1 transcripts/protein inthe wound-edge cohort. USF-1 immunocytochemical staining declinedsignificantly with increasing distance from the denudation site.These data are the first to indicate that binding of USF-1 toits target motif can be induced by `tissue' injury in vitroand implicate USF-1 as a transcriptional regulator of genes (e.g.PAI-1) involved in wound repair.

Key words: Keratinocytes, PAI-1, Reepithelialization, Gene targeting

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