2B] Many of these genes were expressed at even higher levels in

2B]. Many of these genes were expressed at even higher levels in foigr mutant livers (Fig. 2C). In situ hybridization confirmed the enrichment of the UPR target genes bip, chop, and dnajc3 in 5-dpf foigr livers (Fig. 2D, arrow), although moderate induction in other tissues was also found. We found robust xbp1 splicing in 5-dpf foigr livers and, to a lesser extent, in the liverless carcasses of foigr mutants (Fig. 2E) . Although

this website Eif2s1 can be phosphorylated by kinases other than Perk, the marked increase in p-Eif2s1 in 5-dpf foigr mutants (Fig. 2F) suggests Perk activation. The massive up-regulation of each UPR branch and the disruption of the ER structure unequivocally demonstrate that the foigr mutation causes hepatic ER stress. Studies in mice suggest that UPR activation can cause steatosis,6, 9, 10, 29 and acute exposure to TN, which blocks protein glycosylation and induces the UPR, causes steatosis in mice.12, 13 We used TN to determine see more whether ER stress

could cause steatosis in zebrafish. Doses exceeding 2.5 μg/mL were acutely toxic to 3- and 4-dpf larvae, and 2 μg/mL was toxic when larvae were treated for more than 12 hours. Treatment with 1 μg/mL TN from 3 to 5 dpf caused no mortality and only moderate phenotypic abnormalities, including hepatomegaly and steatosis (Fig. 3A,B). The expression of genes required for some hepatic functions was reduced (Fig. Rucaparib molecular weight 3C), and the expression of genes signifying hepatic damage (Fig. 3D) was increased in TN-treated larvae. As expected, prolonged TN treatment induced xbp1 splicing (Fig. 3E) and UPR target genes, including bip and chop (Fig. 3F). These data demonstrate that TN causes ER stress and FLD. Srebps and Atf6 are activated by similar mechanisms involving site 1 and 2 proteases

(encoded by mbtps1 and mbtps2, respectively; see Ye et al.30 and Fig. 4A). Some studies have demonstrated that the UPR and SREBPs are activated together,16-18 whereas others have reported that UPR activation is accompanied by decreased SREBP activation.12, 13, 20, 31 We found that Atf6 depletion induced Srebp2 target genes (Supporting Fig. 2), and this is consistent with the model proposed by Zeng et al.,20 who found that Atf6 suppresses Srebp2 function. Our finding that Srebp2 target genes [3-hydroxy-3-methylglutaryl coenzyme A reductase A (hmgcra) and farnesyl diphosphate farnesyl transferase 1 (fdft1)] were expressed at lower levels in the foigr mutants (Fig. 4B), in which Atf6 was likely activated, supports this hypothesis. Although the genes encoding Srebps or their target genes were mostly unchanged in TN-treated whole larvae, whole foigr mutants, and foigr mutant livers (Fig. 4B), acetyl coenzyme A carboxylase α (acc1) and fatty acid synthase (fasn) were up-regulated in foigr livers.

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