Regulation of mitogen regulated protein/proliferin gene expression in 3T3 cells by basic fibroblast growth factor
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The Department of Biochemistry, Biophysics, and Molecular Biology was founded to give students an understanding of life principles through the understanding of chemical and physical principles. Among these principles are frontiers of biotechnology such as metabolic networking, the structure of hormones and proteins, genomics, and the like.
History
The Department of Biochemistry and Biophysics was founded in 1959, and was administered by the College of Sciences and Humanities (later, College of Liberal Arts & Sciences). In 1979 it became co-administered by the Department of Agriculture (later, College of Agriculture and Life Sciences). In 1998 its name changed to the Department of Biochemistry, Biophysics, and Molecular Biology.
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1959–present
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- Department of Biochemistry and Biophysics (1959–1998)
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- College of Agriculture and Life Sciences (parent college)
- College of Liberal Arts and Sciences (parent college)
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Abstract
Mitogen regulated protein/proliferin (MRP/PLF) is a murine uterine growth factor belonging to the prolactin/growth hormone gene superfamily. Basic fibroblast growth factor (bFGF) regulates its expression in 3T3 cells and is speculated to be among its regulators in vivo. In order to gain insights into its regulation, experiments were performed to elucidate the mechanisms by which bFGF regulates mrp/plf gene expression in 3T3 cells. RT-PCR analyses demonstrated that of the three different forms of MRP/PLF proteins only one, PLF1, is expressed in these cells in response to bFGF. PLF1 could be the product of either plf42 or plf149 genes. bFGF stimulation results in an 8-fold increase in PLF1 mRNA. This increase is not due to transcriptional activation of the plf42 or plf149 genes as evidenced by nuclear run-on in vitro transcription assays as well as by stable transfection analyses of promoters attached to the reporter gene, chloramphenicol acetyl transferase. Northern analyses following treatment of cells with cordycepin, an inhibitor of transcription, and pulse chase analyses of mRNA that was metabolically radiolabeled with 32P-PO4, indicated that PLF1 expression is not regulated at turnover as well. However, radiolabeled pulse chase assays of nuclear RNA demonstrated that bFGF specifically enhances the rate of processing of PLF1 heterogenous nuclear RNA (hnRNA), which accounts for the increase in the PLF1 mRNA in the cytoplasm;One of the three mrp/plf genes, mrp/plf3, was transcriptionally activated by bFGF in stable transfection assays. By performing systematic deletion analyses of the three promoters, we have identified a 10 bp long bFGF response element (FRE) in the mrp/plf3 promoter. DNA gel mobility shift assays revealed that the FRE binds nuclear factors specifically from bFGF-stimulated cells. The corresponding sequence from plf42 and plf149 gene promoters do not exhibit such binding. Nuclear factors recognized by the FRE do not include the AP1 complex. The FRE is active in living cells as evidenced by in vivo competition analyses. Nuclear factors from cells stimulated by other mitogens such as epidermal growth factor, platelet-derived growth factor-aa and phorbol myristate acetate are also recognized by the FRE suggesting that this element may be a general mitogen response element.