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(Received for publication, July
31, 1995; and in revised form, December 6, 1995) Although the liver is the major source of circulating
insulin-like growth factor-I (IGF-I), relatively little is known about
the regulation of IGF-I gene transcription in this tissue. Since
transcripts are initiated largely in exon 1, we established an in
vitro transcription system to evaluate activation of transcription
via the major exon 1 initiation site. Transcription of a G-free
cassette reporter was directed by rat IGF-I genomic fragments, and the
adenovirus major late promoter was used as an internal control. Tissue
specificity was demonstrated by a 60-90% decrease in transcripts
with spleen extracts as compared with liver. 54 base pairs (bp) of
upstream sequence were sufficient to direct IGF-I gene transcription,
and activity increased 5-fold with 300 bp of upstream sequence. DNase I
footprinting revealed four protected regions between -300 and
-60 bp; binding was confirmed by gel shift analysis, and tissue
specificity was demonstrated by reduced shifts with spleen extracts.
The necessity of transcription factor binding to such sites was
established by competition analysis, which revealed a specific decrease
in IGF-I transcription in the presence of a competing fragment. Use of
this in vitro transcription system should permit analysis of
the function of individual transcription factors involved in regulation
of IGF-I gene expression.
Volume 271,
Number 15,
Issue of April 12, 1996 pp. 8667-8674
©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
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