We have previously demonstrated that important regulatory elements responsible for regulated expression of the human GLUT4 promoter are located between -1154 and -412 relative to transcription initiation (Olson, A. L., and Pessin, J. E. (1995) J. Biol. Chem. 270, 23491-23495). Through further analysis of this promoter regulatory region, we have identified a perfectly conserved myocyte enhancer factor 2 (MEF2)-binding domain (-CTAAAAATAG-) that is necessary, but not sufficient, to support tissue-specific expression of a chloramphenicol acetyltransferase reporter gene in transgenic mice. Biochemical analysis of this DNA element demonstrated the formation of a specific DNA-protein complex using nuclear extracts isolated from heart, hindquarter skeletal muscle, and adipose tissue but not from liver. DNA binding studies indicated that this element functionally interacted with the MEF2A and/or MEF2C MADS family of DNA binding transcription factors. MEF2 DNA binding activity was substantially reduced in nuclear extracts isolated from both heart and skeletal muscle of diabetic mice, which correlated with decreased transcription rate of the GLUT4 gene. MEF2 binding activity completely recovered to control levels following insulin treatment. Together these data demonstrated that MEF2 binding activity is necessary for regulation of the GLUT4 gene promoter in muscle and adipose tissue.
Regulation of growth, differentiation, and apoptosis by synthetic retinoids can occur through
mechanisms that are dependent and independent of their ability to bind and activate nuclear
retinoic acid receptors. The objective of this study was to determine if increasing flexibility of
the heteroarotinoid structure would affect the specificity of the synthetic retinoids for the
receptors and for their regulation of cancerous and nonmalignant cells. Methods were developed
to produce the first examples of heteroarotinoids 15a
−
15h, which contain urea and/or thiourea
linking groups between two aryl rings. Substituents at the para position of the single phenyl
ring were either an ester, a nitro group, or a sulfonamide group. Ovarian cancer cell lines
Caov-3, OVCAR-3, SK-OV-3, UCI-101, and 222 were utilized, and the inhibitory prowess of
the heteroarotinoids was referenced to that of 4-HPR (25). Similar to 4-HPR (25), the
heteroarotinoids inhibited growth of all cell lines at micromolar concentrations. Although the
heteroarotinoids did not activate retinoic acid receptors, the agents induced potent growth
inhibition against the cancer cells with weak activity against normal and benign cells. The
growth inhibition was associated with cell loss and induction of reactive oxygen species.
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