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(American Journal of Pathology. 2002;161:471-480.)
© 2002 American Society for Investigative Pathology


Regular Articles

Differential Expression of a Chloride Intracellular Channel Gene, CLIC4, in Transforming Growth Factor-ß1-Mediated Conversion of Fibroblasts to Myofibroblasts

Lone Rønnov-Jessen*, René Villadsen{dagger}, John C. Edwards{ddagger} and Ole W. Petersen{dagger}

From the Zoophysiological Laboratory, the August Krogh Institute,*and the Structural Cell Biology Unit, Department of Medical Anatomy A, the Panum Institute,{dagger}the University of Copenhagen, Copenhagen, Denmark; and St. Louis Veterans Administration Medical Center,{ddagger}St. Louis, Missouri

Conversion of fibroblasts into myofibroblasts as mediated by transforming growth factor-ß1 (TGF-ß1) is the most prominent stromal reaction to a number of epithelial lesions including breast cancer. To identify genes which are regulated during this process, the mRNA profiles from primary breast fibroblasts treated with or without TGF-ß1 were analyzed by differential display. Ninety-five differentially expressed transcripts were PCR-cloned and sequenced, and 28 clones were selected for verification in a hybridization array. By use of gene-specific sequence tags, nine differentially expressed genes were identified. One of the clones, identified as CLIC4, a member of the CLIC family of chloride channels, was up-regulated more than 16 times in myofibroblasts and was therefore chosen for further analysis. Using RT-PCR, comparison with CLIC1, CLIC2, CLIC3, and CLIC5 demonstrated that CLIC4 was unique by being up-regulated by TGF-ß1 in myofibroblasts. Immunohistochemistry showed a hitherto unknown, distinctive pattern of CLIC4 expression in breast stroma. Whereas normal breast fibroblasts were devoid of CLIC4 protein expression, myofibroblasts of breast carcinomas were strongly CLIC4-positive. The functional significance of CLIC4 was analyzed in MEF/3T3 fibroblasts by conditional expression using the tetracycline-repressive gene regulation system. In a migration assay, we found that CLIC4 inhibited cell motility by 27%. These results suggest that CLIC4 is differentially regulated in fibroblasts and that its expression contributes to a collective stationary myofibroblast phenotype.





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