Activation of PPAR{gamma} in colon tumor cell lines by oxidized metabolites of linoleic acid, endogenous ligands for PPAR{gamma}

doi:10.1093/carcin/bgg131

Carcinogenesis Advance Access published online on August 29, 2003
Carcinogenesis, doi:10.1093/carcin/bgg131
© 2003 by Oxford University Press

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CANCER BIOLOGY

Activation of PPAR ${gamma}$ in colon tumor cell lines by oxidized metabolites of linoleic acid, endogenous ligands for PPAR ${gamma}$

Arthur W. Bull ¹^*, Knut R. Steffensen ², Jörg Leers ², and Joseph J. Rafter ³

¹ Oakland University, Department of Chemistry, Rochester, MI 48309-4477
² Center for Biotechnology, Karolinska Institute, NOVUM, 141 86 Huddinge, Sweden
³ Department of Medical Nutrition, Karolinska Institute, NOVUM, 141 86 Huddinge, Sweden

^* Corresponding author. E-mail: abull{at}oakland.edu.

Received 26 November 2002 ; revised 16 July 2003 ; accepted 24 July 2003

Abstract

The nuclear hormone receptor peroxisome proliferator-activatedreceptor (PPAR) ${gamma}$ plays an important role in the differentiationof intestinal cells and other tissues. Real time PCR examinationof PPAR mRNA for ${gamma}$ 1, 2, and 3, in Caco-2 and HCT-116 colon celllines showed that ${gamma}$ 3 is the most abundant message in both lines.Treatment of Caco-2 cells with sodium butyrate, which inducescell differentiation, also leads to an increase in all threePPAR mRNAs. In contrast, treatment of HCT-116 cells with sodiumbutyrate, which does not lead to differentiation of these cells,causes a decrease in the amount of all three PPAR mRNAs. Furthermore,the amount of PPAR mRNA is greater in Caco-2 cells than in HCT-116cells at all times examined.

Since several oxidative metabolitesof linoleic acid, including 13-hydroxyoctadecadienoic acid (13-HODE)and 13-oxooctadecadienoic acid (13-OXO) have been shown to bindPPAR, and there is a strong positive correlation between enzymesfor metabolism of linoleate oxidation products, intestinal celldifferentiation, and the distribution of PPAR, we also performeda detailed investigation of the activation of PPAR ${gamma}$ by 13-HODEand 13-OXO. For these experiments, Caco-2 and HCT-116 cellswere transfected with constructs containing PPAR ${gamma}$ 1 or ${gamma}$ 2 thena PPRE-luc reporter construct. Exposure of transfected cellsto micromolar concentrations of 13-HODE or 13-OXO produced concentrationdependent increases in luciferase activity. In addition, thetwo linoleate metabolites activate endogenous PPAR in thesecell lines transfected with only PPRE-luc. These data substantiatethe contention that oxidation products of linoleic acid aremetabolically produced endogenous ligands for PPAR ${gamma}$ and thatPPAR ${gamma}$ plays an important role in the differentiation of intestinalcells.

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Carcinogenesis

Activation of PPAR in colon tumor cell lines by oxidized metabolites of linoleic acid, endogenous ligands for PPAR

Activation of PPAR ${gamma}$ in colon tumor cell lines by oxidized metabolites of linoleic acid, endogenous ligands for PPAR ${gamma}$