Am. J. Respir. Cell Mol. Biol., Vol 14, No. 2, 02 1996, 121-130.
Characterization of the human surfactant protein D promoter: transcriptional regulation of SP-D gene expression by glucocorticoids
K Rust, L Bingle, W Mariencheck, A Persson and EC Crouch
Department of Pathology, Washington University School of Medicine, St. Louis, Missouri 63110, USA.
We have previously described the characterization of genomic clones
encoding the entire translated sequence of human pulmonary surfactant
protein D (SP-D). We now describe the characterization of a genomic
fragment (H5E7) that encodes the entirety of the first translated exon
(Exon 2), Intron 1, a short transcribed untranslated sequence (Exon 1; 39
bp), and approximately 4 kb of sequence upstream from the transcription
initiation site. The start site was identified by 5'-RACE- PCR cloning and
primer extension. A putative TATA box (CATAAATA) was identified
approximately 30 bp upstream of the start site. Complete sequencing of a
HindIII/SacI fragment (HS-1674) encoding approximately 1.7 kb of sequence
5' to the TATA demonstrated multiple potential cis- regulatory elements
including half-site glucocorticoid response elements (GRE), a canonical
AP-1 consensus, several AP-1 like sequences, E-box sequences, NF-IL-6 and
PEA3 motifs, and putative interferon response elements. H441 lung
adenocarcinoma cells, which express low levels of SP-D mRNA, and liver
HepG2 cells, were transiently co-transfected with chloramphenicol acetyl
transferase (CAT) reporter constructs containing up to 3,000 base pairs of
upstream sequence, and with constructs encoding beta-gal. H441 cells
transfected with constructs containing at least 161 bp of upstream sequence
gave normalized levels of CAT activity greater than or equal to that
obtained for parallel positive control transfections using pTK-CAT.
Treatment of the cells for 48 h with 50 nM dexamethasone (Dex) gave a 2- to
5-fold increase in CAT activity. Interestingly, a 5'-deletion construct
containing 161 bp of upstream sequence (pFS161-CAT) conferred both cell
type-restricted and dexamethasone-responsive expression. These studies
emphasize the potential complexity of SP-D gene regulation, and further
support the hypothesis that the effects of glucocorticoids on SP-D
production in vivo are regulated at the level of transcription.
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Copyright © 1996 American Thoracic Society.
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