Developmental and glucocorticoid regulation of surfactant protein mRNAs in preterm lambs

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Am J Physiol Lung Cell Mol Physiol 277: L1142-L1148, 1999;
1040-0605/99 $5.00

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Vol. 277, Issue 6, L1142-L1148, December 1999

Developmental and glucocorticoid regulation of surfactant protein mRNAs in preterm lambs

Rosemarie C. Tan¹, Machiko Ikegami², Alan H. Jobe², Li Yuan Yao³, Fred Possmayer³, and Philip L. Ballard¹

¹ Department of Pediatrics, University of Pennsylvania School of Medicine, Children's Hospital of Philadelphia, Philadelphia, Pennsylvania 19104; ² Pulmonary Biology, Children's Hospital Medical Center, Cincinnati, Ohio 45229; and ³ Department of Obstetrics and Gynecology and Biochemistry, Lawson Research Institute, St. Joseph's Health Centre and London Health Sciences Centre, University Campus, University of Western Ontario, London, Ontario, Canada N6A 4V2

Glucocorticoid treatment increases content of surfactant protein (SP) A and SP-B in lung tissue and lavage fluid of pretermlambs. To investigate this process, we determined the ontogenyand glucocorticoid induction of SP mRNAs. In separate treatmentprotocols, each with its own controls, sheep were injected withbetamethasone 15 h, 48 h, or weekly for 1-4 doses before pretermdelivery. Using ovine SP cDNAs, we found an increase equal toor more than threefold in basal levels of all three SP mRNAs between125 days and term. After betamethasone treatment, SP-B and SP-CmRNA levels increased by 15 h and all SP mRNAs were elevated after24 h ( $>=$ 2-fold); mRNA levels in fetuses delivered 1-3 wk afterbetamethasone were not different from control. We conclude thatin vivo betamethasone rapidly induces a coordinated increase inSP mRNAs, which is fully reversible within 7 days despite repetitivedoses of betamethasone. Similar increases in mRNA and proteincontents for SP-A and SP-B suggest that glucocorticoid regulationof these SPs in vivo is primarilypretranslational.

betamethasone; ontogeny

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