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1 Institute for Environmental Medicine, University of Pennsylvania School of Medicine, Philadelphia 19104-6068; and Departments of 2 Pathology and 3 Molecular Pharmacology, MCP Hahnemann University School of Medicine, Philadelphia, Pennsylvania 19129
Surfactant protein A (SP-A) is expressed in lung
alveolar type II cells and bronchiolar Clara cells. We have identified
two active regions in the promoter of the rat SP-A gene by deletion analysis of a plasmid containing 163 bp before the start of
transcription (
163 bp), linked to a reporter gene. Constructs
were transfected into lung cell lines derived from each of the cell
types that produces SP-A. We found a novel region of promoter activity
at ~90 bp before the transcriptional start (SP-A
90).
Mutation of four nucleotides in SP-A
90 that are
highly conserved among species (
92 to
89 bp) decreased
expression of the SP-A construct by ~50% in both cell lines.
Electrophoretic mobility shift analysis showed specific binding to
SP-A
90 by nuclear proteins from the cell lines, as
well as from rat lung and liver. The electrophoretic mobility of the
bands shifted by lung nuclear proteins changed late in fetal
development. Although in the Clara cell line no reduction of promoter
activity was seen on deletion of the region upstream of
SP-A
90, in the type II cell line, deletion of
residues
163 to
133 did reduce activity by ~50%. This
region contains a recognition element for thyroid transcription factor-1 (TTF-1). Endogenous TTF-1 binding activity was substantially higher in the type II cell line than in the Clara cell line, but cotransfection of a TTF-1 expression plasmid enhanced expression of the
SP-A construct better in the Clara cell line than in the type II cell
line. These results suggest that the recognition element for TTF-1 has
varying activity in the lung cell lines of different origin due to the
availability of TTF-1.
gene regulation; transcription factors; lung development; NCI-H441 cells; MLE-15 cells
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