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Penn Center for the Molecular Studies of Kidney Diseases, University of Pennsylvania, Philadelphia, Pennsylvania 19104-6144
The
FSP1 gene encodes a filament-binding
S100 protein with paired EF hands that is specifically
expressed in fibroblasts. This led us to look for
cis-acting elements in the
FSP1 promoter that might engage
nuclear transcription factors unique to fibroblasts. The first exon of
FSP1 is noncoding, therefore, a series of luciferase reporter minigenes
were created containing varying lengths of 5'-flanking sequence,
the first intron, and the noncoding region of the second exon. A
position and promoter-dependent proximal element between
187 and
88 bp was shown to be active in fibroblasts but not in
epithelium. Sequence in the first intron from +777 to +964 had an
enhancing effect that was not cell type specific. Hsv
TK reporter constructs driven by this promoter/intron
cassette in transgenic mice were coexpressed appropriately with FSP1 in tissue fibroblasts. Gel mobility shift competitor assays identified a
novel domain, FTS-1 (fibroblast transcription site-1; TTGAT from
177 to
173 bp), that specifically interacts with nuclear extracts from fibroblasts. The necessity of this binding
site was confirmed by site-specific mutagenesis. Database searches also
turned up putative FTS-1 sites in the early promoter regions of other
fibroblast expressed proteins, including the
1 and
2(I), and
1(III) collagens
and the
SM-actin gene. We hypothesize that the
selective engagement of FTS-1 elements may contribute to
the mesenchymal phenotype of fibroblasts and perhaps other
dedifferentiated cells.
FSP1; fibroblast; transcription; cis-acting element
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