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JCS ePress online publication date 31 Jul 2007
doi: 10.1242/jcs.03480


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Research Article

Reduced migration, altered matrix and enhanced TGF{beta}1 signaling are signatures of mouse keratinocytes lacking Sdc1


Mary Ann Stepp*, Yueyuan Liu, Sonali Pal-Ghosh, Rosalyn A. Jurjus, Gauri Tadvalkar, Adith Sekaran, Kristen LoSicco, Li Jiang, Melinda Larsen, Luowei Li, and Stuart H. Yuspa
* Author for correspondence (e-mail: mastepp{at}gwu.edu)

We have reported previously that syndecan-1 (Sdc1)-null mice show delayed re-epithelialization after skin and corneal wounding. Here, we show that primary keratinocytes obtained from Sdc1-null mice and grown for 3-5 days in culture are more proliferative, more adherent and migrate more slowly than wt keratinocytes. However, the migration rates of Sdc1-null keratinocytes can be restored to wild-type levels by replating Sdc1-null keratinocytes onto tissue culture plates coated with fibronectin and collagen I, laminin (LN)-332 or onto the matrices produced by wild-type cells. Migration rates can also be restored by treating Sdc1-null keratinocytes with antibodies that block {alpha}6 or {alpha}v integrin function, or with TGF{beta}1. Antagonizing either {beta}1 integrin function using a function-blocking antibody or TGF{beta}1 using a neutralizing antibody reduced wild-type keratinocyte migration more than Sdc1-null keratinocyte migration. Cultures of Sdc1-null keratinocytes accumulated less collagen than wild-type cultures but their matrices contained the same amount of LN-332. The Sdc1-null keratinocytes expressed similar total amounts of eight different integrin subunits but showed increased surface expression of {alpha}v{beta}6, {alpha}v{beta}8, and {alpha}6{beta}4 integrins compared with wild-type keratinocytes. Whereas wild-type keratinocytes increased their surface expression of {alpha}2{beta}1, {alpha}v{beta}6, {alpha}v{beta}8, and {alpha}6{beta}4 after treatment with TGF{beta}1, Sdc1-null keratinocytes did not. Additional data from a dual-reporter assay and quantification of phosphorylated Smad2 show that TGF{beta}1 signaling is constitutively elevated in Sdc1-null keratinocytes. Thus, our results identify TGF{beta}1 signaling and Sdc1 expression as important factors regulating integrin surface expression, activity and migration in keratinocyte and provide new insight into the functions regulated by Sdc1.




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