Hepatic ATGL mediates PPAR-α signaling and fatty acid channeling through an L-FABP independent mechanism

Kuok Teong Ong,Mara T Mashek,Nicholas O Davidson,Douglas G Mashek

doi:10.1194/jlr.m039867

Kuok Teong Ong, Mara T Mashek + Show 2 more

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https://doi.org/10.1194/jlr.m039867

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Adipose TG lipase (ATGL) catalyzes the rate-limiting step in TG hydrolysis in most tissues. We have shown that hepatic ATGL preferentially channels hydrolyzed FAs to β-oxidation and induces PPAR-α signaling. Previous studies have suggested that liver FA binding protein (L-FABP) transports FAs from lipid droplets to the nucleus for ligand delivery and to the mitochondria for β-oxidation. To determine if L-FABP is involved in ATGL-mediated FA channeling, we used adenovirus-mediated suppression or overexpression of hepatic ATGL in either WT or L-FABP KO mice. Hepatic ATGL knockdown increased liver weight and TG content of overnight fasted mice regardless of genotype. L-FABP deletion did not impair the effects of ATGL overexpression on the oxidation of hydrolyzed FAs in primary hepatocyte cultures or on serum β-hydroxybutyrate concentrations in vivo. Moreover, L-FABP deletion did not influence the effects of ATGL knockdown or overexpression on PPAR-α target gene expression. Taken together, we conclude that L-FABP is not required to channel ATGL-hydrolyzed FAs to mitochondria for β-oxidation or the nucleus for PPAR-α regulation.

Highlights

Adipose TG lipase (ATGL) catalyzes the rate-limiting step in TG hydrolysis in most tissues
ATGL knockdown had no effect on body weight in WT or liver FA binding protein (L-FABP) KO mice when compared with control shRNA treatment (Fig. 1B)
ATGL knockdown led to increased liver weight in WT mice and this effect was replicated in L-FABP KO mice (Fig. 1C)

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Introduction

Adipose TG lipase (ATGL) catalyzes the rate-limiting step in TG hydrolysis in most tissues. We have shown that hepatic ATGL selectively channels hydrolyzes FAs to ␤-oxidation without affecting VLDL secretion [1]. We have shown that the expression of PPAR-␣ and its downstream target genes is decreased in mice or primary hepatocytes receiving ATGL shRNA [1]. These results are consistent with microarray analysis of tissues in the whole-body ATGL KO mice [7] and work from others reporting that ATGL regulates PPAR-␣ in heart, small intestine, and brown adipose tissue [4,5,6]. Data defining the mechanism through which ATGL regulates PPAR-␣ or how FAs are trafficked to PPAR-␣ are lacking

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