Correlation between riboflavin carrier protein induction and its mRNA activity in estrogen stimulated chicken liver and oviduct

Durga Kumari, B. ; Adiga, P. R. (1986) Correlation between riboflavin carrier protein induction and its mRNA activity in estrogen stimulated chicken liver and oviduct Journal of Biosciences, 10 (2). pp. 193-202. ISSN 0250-5991

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Official URL: http://www.ias.ac.in/jarch/jbiosci/10/193-202.pdf

Related URL: http://dx.doi.org/10.1007/BF02703477

Abstract

Poly A enriched RNA from either liver or oviduct of estradiol-17β treated immature chicks supported [3H]-leucine incorporation into immunoprecipitable riboflavin carrier protein in a dose-dependent manner when translated in the rabbit reticulocyte lysate system. Primary translation product of riboflavin carrier protein had a molecular weight of 38,000 which on incubation with a stripped hepatic microsomal preparation was processed to a product with a size comparable to native riboflavin carrier protein. Poly A enriched RNA from both the liver and the oviduct of estrogen-treated birds stimulated [3H]-leucine incorporation into riboflavin carrier protein and this was 2-3 fold higher during secondary stimulation vis-a-vis primary stimulation with the steroid. Poly A enriched RNA from the liver of progesteronetreated birds during secondary stimulation did not support riboflavin carrier protein synthesis. In contrast, poly A enriched RNA from the oviduct of the birds treated with progesterone during secondary (but not primary) stimulation did exhibit riboflavin carrier protein-mRNA activity which was comparable to that stimulated by estradiol-17β.

Item Type:Article
Source:Copyright of this article belongs to Indian Academy of Sciences.
Keywords:Primary Translation Product; Cell-free Translation; Rabbit Reticulocyte Lysate; Stripped Microsomal Membrane; Progesterone; Estradiol-17β Precursor; Poly A+-RNA
ID Code:26758
Deposited On:08 Dec 2010 13:14
Last Modified:17 May 2016 10:03

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