Your search keyword '"MacIntyre SS"' showing total 2 results

1. Studies of translatable mRNA for rabbit C-reactive protein.

Author

Samols D, MacIntyre SS, and Kushner I

Subjects

Animals, Cell-Free System, Chemical Precipitation, Electrophoresis, Polyacrylamide Gel, Methylmercury Compounds pharmacology, Protein Denaturation drug effects, Rabbits, Reticulocytes metabolism, C-Reactive Protein genetics, Protein Biosynthesis drug effects, RNA, Messenger genetics

Abstract

C-reactive protein (CRP) mRNA was assayed by cell-free translation of poly(A)-containing liver RNA isolated both from rabbits stimulated to undergo the acute-phase response and from unstimulated control rabbits. No CRP-related translation products were identified until the denaturant methylmercury hydroxide (CH3HgOH) was added to the RNA before cell-free translation. In the presence of the denaturant, a 24000-Da translation product was synthesized which was immunochemically identifiable as the CRP primary translation product. It is likely that rabbit CRP mRNA can form a stable intramolecular duplex which interferes with its translatability in vitro. The 24000-Da CH3HgOH-facilitated cell-free translation product was not detected in poly(A)-containing liver RNA from unstimulated animals, indicating that the concentration of translatable CRP mRNA was dramatically induced during the acute-phase response. On the basis of absorption experiments, the 24000-Da CRP primary translation product was immunochemically more closely related to denatured CRP than to native CRP.

Published

1985

2. Synthesis and secretion of C-reactive protein by rabbit primary hepatocyte cultures.

Author

MacIntyre SS, Schultz D, and Kushner I

Subjects

Animals, C-Reactive Protein biosynthesis, Cells, Cultured, Electrophoresis, Polyacrylamide Gel, Inflammation metabolism, Kinetics, Liver cytology, Rabbits, Radioimmunoassay, C-Reactive Protein metabolism, Liver metabolism

Abstract

The synthesis and secretion of the acute-phase protein C-reactive protein by rabbit primary hepatocyte cultures was investigated. Hepatocytes prepared from animals that had received inflammatory stimuli 18-24 h before cell isolation were found to incorporate radiolabelled amino acids into C-reactive protein throughout the 48 h culture period. Intracellular C-reactive protein was found to be in steady state and there was no significant degradation of extracellular C-reactive protein, permitting direct estimation of rate of synthesis from rate of extracellular accumulation. Both C-reactive protein and total secreted protein were synthesized at constant rates for at least 24 h in culture. Mean rate of accumulation of newly synthesized total proteins in medium of cultures from six stimulated animals was 40% greater than was found in cultures from nine control (unstimulated) animals; this difference did not achieve statistical significance (0.05 less than P less than 0.10). Mean rate of C-reactive-protein synthesis represented 3.9% of total secreted-protein synthesis in cultures prepared from stimulated animals compared with 0.3% in cultures from control animals (P less than 0.001). Further, there was a correlation between C-reactive-protein synthesis by cultured hepatocytes and serum C-reactive-protein concentration at time of hepatocyte isolation (P less than 0.001). Rates of C-reactive-protein synthesis by hepatocyte cultures from stimulated animals were in good agreement with those previously measured in isolated perfused livers and those calculated from results of studies in vivo.

Published

1983