Matrix Gla protein mRNA expression in cultured type II pneumocytes. | - CCMAR -

Journal Article

TitleMatrix Gla protein mRNA expression in cultured type II pneumocytes.
Publication TypeJournal Article
AuthorsRannels, SR, M. Cancela, L, Wolpert, EB, Price, PA
Year of Publication1993
JournalAm J Physiol
Volume265
Issue3 Pt 1
Date Published1993 Sep
PaginationL270-8
ISSN0002-9513
KeywordsAnimals, Blotting, Northern, Carbon-Carbon Ligases, Cells, Cultured, Extracellular Matrix, Ligases, Lung, Male, Osteocalcin, Rats, Rats, Sprague-Dawley, RNA, Messenger, Tretinoin, Vitamin K Deficiency
Abstract

Matrix Gla protein (MGP) was first isolated from the matrix fraction of bone. This highly conserved vitamin K-dependent protein of 14 kDa has been identified in numerous tissues and cells, and its mRNA was recently found to be abundant in rat lung. Relatively low MGP protein levels in many soft tissues where its mRNA is high suggests an important secretory function for this protein. We have found a high specific activity of vitamin K-dependent carboxylase in microsomes of rat pulmonary type II cells and the presence of numerous endogenous substrates, including one of 13-15 kDa. To investigate the possibility that MGP and its mRNA could be localized in type II cells, rat MGP and actin cDNA probes were hybridized to total RNA obtained from freshly isolated type II cells and from cells cultured for up to 6 days. MGP mRNA increased 5- to 6-fold relative to beta-actin mRNA from days 3 to 6 in primary culture and MGP secretion increased nearly 60-fold during that interval. MGP mRNA and MGP secretion decreased 25-75% if cultures were supplemented with vitamin K quinone. Vitamin K deficiency, caused by carbon stripping the serum or treatment of cell cultures with warfarin, resulted in an induction of carboxylase activity and elevated MGP mRNA. In parallel experiments, carboxylase specific activity also increased during culture in the presence or absence of vitamin K. Retinoic acid further increased steady-state mRNA levels and MGP secretion at later culture intervals, an effect which was serum dependent.(ABSTRACT TRUNCATED AT 250 WORDS)

Sapientia

http://www.ncbi.nlm.nih.gov/pubmed/8214087?dopt=Abstract

Alternate JournalAm. J. Physiol.
PubMed ID8214087
Grant ListAR-25921 / AR / NIAMS NIH HHS / United States
HL-42482 / HL / NHLBI NIH HHS / United States
CCMAR Authors