Data on regulation of the gene for the adipocyte-enriched micropeptide Adig/Smaf1 by qPCR analysis and luciferase reporter assay

Gang Ren; Nicholas Cairl; Ji Young Kim; Cynthia M Smas

doi:10.1016/j.dib.2016.09.034

Data on regulation of the gene for the adipocyte-enriched micropeptide Adig/Smaf1 by qPCR analysis and luciferase reporter assay

Data Brief. 2016 Sep 24:9:635-641. doi: 10.1016/j.dib.2016.09.034. eCollection 2016 Dec.

Authors

Gang Ren¹, Nicholas Cairl¹, Ji Young Kim¹, Cynthia M Smas¹

Affiliation

¹ University of Toledo College of Medicine, Department of Biochemistry and Cancer Biology and the Center for Diabetes and Endocrine Research, Toledo, OH, USA.

Abstract

This article describes qPCR analysis for the Adig/Smaf1 gene in multiple in vitro adipocyte differentiation models including white and brown adipogenesis, cell lines and primary cultures. The article also contains qPCR data for transcript levels of Adig/Smaf1 in a wide panel of murine tissues. Expression of Adig/Smaf1 transcript in white and brown adipose tissue in fasted and refed mice is reported and also data for Adig/Smaf1 transcript expression in genetically obese ob/ob mice. Data on the effects of siRNA-mediated knockdown of Srebp1c on Adig/Smaf1 transcript levels in 3T3-L1 adipocytes are shown. Luciferase reporter assays provide data for regulation of an ~ 2 kb fragment of the 5' flanking region of Adig/Smaf1 gene by PPARγ/RXRα. This data is related to a research article describing Adig/Smaf1 protein expression, "Expression, regulation and functional assessment of the 80 amino acid Small Adipocyte Factor 1 (Smaf1) protein in adipocytes" (G. Ren, P. Eskandari, S. Wang, C.M. Smas, 2016) [1].

Keywords: Adipocyte; Adipogenesis; Adipose tissue; Nutritional regulation, Obesity; PPARgamma.