Functional characterization of the L-type pyruvate kinase gene glucose response complex.

Guerra, Matt; Bergot, M O; Martinez, Antoine; Cuif, Marie Hélène; Kahn, Axel; Raymondjean, Michel

doi:10.1128/mcb.13.12.7725

Cited by 111 publications

(112 citation statements)

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“…A number of studies have established that FKHR activates the transcription of gluconeogenic enzymes in the absence of insulin and inhibits the transcription in the presence of insulin. On the other hand, HNF-4 positively regulates the genes involved in glucose transport and glycolysis (4,6). Here, we provided a novel mechanism that insulin reversed the repression of HNF-4 transcriptional activity by FKHR.…”

Section: Effects Of Insulin On the Repression Of Hnf-4 Transactivatiomentioning

confidence: 81%

Hepatocyte Nuclear Factor-4 Is a Novel Downstream Target of Insulin via FKHR as a Signal-regulated Transcriptional Inhibitor

Hirota

Daitoku

Matsuzaki

et al. 2003

Journal of Biological Chemistry

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HNF-4, 1 a member of the steroid/thyroid nuclear receptor superfamily, is a transcriptional factor which expresses in the liver, intestine, kidney, and pancreatic ␤-cells (1, 2). It contains several functional domains: a ligand-independent activation domain (AF1), a zinc finger DNA binding domain, and a ligand-dependent activation domain (AF2) (3). HNF-4 binds to a specific DNA element as a homodimer and regulates the expression of many genes, involved in glucose, fatty acid, and cholesterol metabolisms (4 -6). The blood glucose levels are controlled by the balance of two opposing hormones, glucagon and insulin. Whereas glucagon decreases the activity of HNF-4, the effect of insulin on that of HNF-4 has not fully been understood yet (7-9).FKHR, a forkhead family member, is a transcriptional factor and regulates the expression of multiple genes, such as key enzymes of gluconeogenesis (10, 11). Insulin has a dynamic effect on the localization of FKHR, when phosphorylated by Akt at the three residues of FKHR: Thr-24, Ser-253, and Ser-316. Once phosphorylated, the cytoplasmic retention is induced, leading to inhibit the transcriptional activity. On the other hand, in the absence of insulin, FKHR is dephosphorylated and localized to the nucleus, where FKHR binds to the specific DNA element, resulting in transcriptional activation of the target genes (12-15).Recently, it has been reported that FKHR activates or represses the transactivation by nuclear receptor family members as a DNA binding-independent cofactor (16,17). In the present study, we analyzed the interaction of FKHR with HNF-4, the effect of FKHR on the transactivation mediated by HNF-4, and its molecular mechanism. FKHR associates with HNF-4 in vivo and in vitro and represses the transactivation by HNF-4 through the decrease in its DNA binding affinity. Interestingly, the inhibitory effect is canceled by insulin, resulting from the dissociation of HNF-4 from phosphorylated FKHR that subsequently translocates to the cytoplasm. This suggests the possibility that HNF-4 is a novel downstream target of insulin via FKHR as a signal-regulated transcriptional inhibitor. EXPERIMENTAL PROCEDURESCell Culture and Transfections and Reporter Gene Assays-HepG2 cells were cultured in Dalbecco's modified Eagle's medium supplemented with 10% fetal bovine serum. Transfections were performed by FuGENE-6 (Roche Molecular Biochemicals). Twenty ng of pCMV-␤gal plasmid were included in each transfection experiment to control for the efficiency of transfection. To ensure equal DNA amounts, empty plasmids were added in each transfection. The luciferase activity was measured with an ARVO™SX (Wallac Berthold). The values were normalized to ␤-galactosidase activity as an internal control.Plasmids-The hHNF-4 ␣2 cDNA was subcloned into pcDNA3 tagged with the HA epitope (pcDNA3HA). A series of HNF-4 deletion fragments were generated by PCR and subcloned into pGEX 4T-1 (Amersham Biosciences) or pcDNA3HA. The pGAL4-HNF-4 vector was made by subcloning hHNF-4 ␣2 cDNA tagged with the Gal4 DN...

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Section: Effects Of Insulin On the Repression Of Hnf-4 Transactivatiomentioning

confidence: 81%

Hepatocyte Nuclear Factor-4 Is a Novel Downstream Target of Insulin via FKHR as a Signal-regulated Transcriptional Inhibitor

Hirota

Daitoku

Matsuzaki

et al. 2003

Journal of Biological Chemistry

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“…The promoter (-183 to +11) contains binding sites for HNF-1, NF-I, HNF-4, upstream stimulating factor (USF)-related proteins and L5-binding factors (Figure 1) [80][81][82][83]. The HNF-4 site also binds chicken ovalbumin upstream promoter-transcription factor (COUP-TF)I and COUP-TFII [84]. The binding of HNF-4 apparently stabilizes NF-I binding [80].…”

Section: Tissue-specific Controlmentioning

confidence: 99%

Transcriptional control of genes that regulate glycolysis and gluconeogenesis in adult liver

Lemaigre¹,

Rousseau²

1994

Biochemical Journal

100

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“…ChREBP is reported to bind to L-III as a heterodimer with Max-like protein X. It has been widely accepted that HNF4␣ is involved in transcriptional activation of the L-PK gene, because reporter gene assays and binding assays showed that HNF4␣ stimulates the L-PK promoter activity by binding to the L-IIB element (10,13,24). However, we suspected an alternative mechanism, because NF1 family members also bind to the L-IIB element as well as the accessory element in the S 14 gene, whereas HNF4␣ does not bind to this element in the S 14 gene (25).…”

mentioning

confidence: 99%

Nuclear Factor 1 Family Members Interact with Hepatocyte Nuclear Factor 1α to Synergistically Activate L-type Pyruvate Kinase Gene Transcription

Satoh

Noaki

Ishigure

et al. 2005

Journal of Biological Chemistry

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Transcription of hepatic L-type pyruvate kinase (L-PK) gene is cell type-specific and is under the control of various nutritional conditions. The L-PK gene contains multiple cis-regulatory elements located within a 170-bp upstream region necessary for these regulations. These elements can synergistically stimulate L-PK gene transcription, although their mechanisms are largely unknown. Because nuclear factor (NF) 1 family members bind to specific cisregulatory elements known as L-IIA and L-IIB and hepatocyte nuclear factor (HNF) 1␣ binds to the adjacent element L-I, we examined the functional and physical interactions between these two transcription factors. Reporter gene assay showed that these two factors synergistically activated the L-PK promoter containing the 5-flanking region up to ؊189. Although two NF1-binding sites are required for the maximum synergistic effect of NF1 family members with HNF1␣, significant functional interaction between the two factors was observed in the L-PK promoter containing two mutated NF1-binding sites and also in the promoter containing only the HNF1␣-binding site, raising the possibility that NF1 proteins function as HNF1␣ co-activators. Chromatin immunoprecipitation assay revealed that both NF1 proteins and HNF1␣ bound to the promoter region of the L-PK gene in vivo. In vitro binding assay confirmed that NF1 proteins directly interacted mainly with the homeodomain of HNF1␣ via their DNA-binding domains. This interaction enhanced HNF1␣ binding to the L-I element and was also observed in rat liver by co-immunoprecipitation assay. Thus, we conclude that cooperative interaction between NF1 family members and HNF1␣ plays an important role in hepatic L-PK transcription.Pyruvate kinase (ATP, pyruvate 2-O-phosphotransferase; PK) 2 is an important regulatory enzyme in the glycolytic pathway. Four PK isozymes are known to exist in mammals and are designated as L, R, M 1 , and M 2 types (1). They are produced from two genes, PKL and PKM, by alternative use of two promoters and mutually exclusive alternative splicing, respectively (2-4). The L-type isozyme (L-PK) is expressed in a tissue-specific manner; this form is expressed primarily in hepatic parenchymal cells and is also present in pancreatic ␤ cells, kidney, and small intestine (1). Hepatic L-PK gene expression is also transcriptionally controlled positively by glucose in the presence of insulin and negatively by polyunsaturated fatty acids or glucagon via cyclic AMP (5-8). These regulations of the L-PK gene transcription are mediated via the multiple cis-regulatory elements located within a 170-bp upstream region from the transcription start site, as shown in Fig. 1 (8 -10). We have named these elements L-I (Ϫ94 to Ϫ76), L-II (Ϫ149 to Ϫ126), and L-III (Ϫ170 to Ϫ150) (9). In addition, another group has identified a weak negative element (Ϫ116 to Ϫ99) between L-I and L-II (10). Although this element has been named L2, we will refer to this as L-IIA and L-II as L-IIB hereafter. Although L-IIB is considered to be a regulatory element...

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Functional characterization of the L-type pyruvate kinase gene glucose response complex.

Cited by 111 publications

References 32 publications

Hepatocyte Nuclear Factor-4 Is a Novel Downstream Target of Insulin via FKHR as a Signal-regulated Transcriptional Inhibitor

Hepatocyte Nuclear Factor-4 Is a Novel Downstream Target of Insulin via FKHR as a Signal-regulated Transcriptional Inhibitor

Transcriptional control of genes that regulate glycolysis and gluconeogenesis in adult liver

Nuclear Factor 1 Family Members Interact with Hepatocyte Nuclear Factor 1α to Synergistically Activate L-type Pyruvate Kinase Gene Transcription

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