AI Article Synopsis

  • CACT is an important protein that helps transport long-chain fatty acids into mitochondria for energy production, and this study focuses on how its gene regulation is affected by omega-3 fatty acids (EPA and DHA).
  • In liver cells, EPA and DHA were found to increase the levels of CACT mRNA and protein, highlighting their role in promoting this gene's expression.
  • The research identified a specific region in the CACT promoter that responds to n-3 PUFAs, involving GABP proteins rather than PPARα, suggesting that GABP may play a key role in the activation of the CACT gene by these fatty acids.

Article Abstract

Carnitine-acylcarnitine translocase (CACT) is a nuclear-encoded mitochondrial carrier that catalyzes the transfer of long-chain fatty acids across the inner mitochondrial membrane for β-oxidation. In this study, we conducted a structural and functional characterization of the CACT promoter to investigate the molecular mechanism underlying the transcriptional regulation of the CACT gene by n-3 PUFA, EPA and DHA. In hepatic BRL3A cells, EPA and DHA stimulate CACT mRNA and protein expression. Deletion promoter analysis using a luciferase reporter gene assay identified a n-3 PUFA response region extending from -202 to -29 bp. This region did not contain a response element for PPARα, a well-known PUFA-responsive nuclear receptor. Instead, bioinformatic analysis revealed two highly conserved GABP responsive elements within this region. Overexpression of GABPα and GABPβ subunits, but not PPARα, increased CACT promoter activity, more remarkably upon treatment with EPA and DHA. ChIP assays showed that n3-PUFA enhanced the binding of GABPα to the -202/-29 bp sequence. Furthermore, both EPA and DHA induced nuclear accumulation of GABPα. In conclusion, our findings indicate that the upregulation of CACT by n3-PUFA in hepatic cells is independent from PPARα and could be mediated by GABP activation.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC11354350PMC
http://dx.doi.org/10.3390/ijms25169095DOI Listing

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