Transcriptional Regulation of α1b Adrenergic Receptors (α1bAR) by Nuclear Factor 1 (NF1): a Decline in the Concentration of NF1 Correlates with the Downregulation of α1bAR Gene Expression in Regenerating Liver

Gao, Bin; Liu, Jiang; Kunos, George

doi:10.1128/mcb.16.11.5997

Cited by 50 publications

(49 citation statements)

References 56 publications

(79 reference statements)

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“…Studies of adrenergic receptor expression in the liver show that, based on the proliferative state of the hepatocyte, alphaand beta-adrenergic GPCRs are differentially expressed. 31,32 Similar changes in adrenergic receptor expression are observed when hepatocytes are placed into primary culture. The expression of multiple other proteins, such as the Ntcp bile acid transporter, cytochrome P450 enzymes, also changes during the primary culture of hepatocytes and in established cell lines.…”

Section: Discussionmentioning

confidence: 55%

Conjugated bile acids promote ERK1/2 and AKT activation via a pertussis toxin-sensitive mechanism in murine and human hepatocytes

et al. 2005

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Section: Discussionmentioning

confidence: 55%

Conjugated bile acids promote ERK1/2 and AKT activation via a pertussis toxin-sensitive mechanism in murine and human hepatocytes

et al. 2005

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“…The mixtures were analyzed by DNA gel mobility shift assay using 32 P-labeled oligo II as a probe. 1 MF-2 Cells, Respectively-Our previous data showed that NF1/L, NF1/Red1, and NF1/X were able to activate transcription via the P2 promoter to more or less the same degree in Hep3B cells as in primary cultured hepatocytes (8). We wondered whether these NF1 isoforms can also regulate the P2 promoter activity in DDT 1 MF-2 smooth muscle cells.…”

Section: Methodsmentioning

confidence: 99%

“…Construction of Plasmids-The pNF1/X, pNF1/Red1, and pNF1/L expression vectors were prepared as described previously (8). The deleted NF1 expression vectors are prepared by subcloning the cDNAs encoding a set of truncated NF1 proteins into pcDNA3 expression vectors.…”

Section: Methodsmentioning

confidence: 99%

Cell type-specific Transcriptional Activation and Suppression of the α1B Adrenergic Receptor Gene Middle Promoter by Nuclear Factor 1

Gao

Kunos

1998

Journal of Biological Chemistry

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Nuclear factor 1 (NF1) has been reported to be a transcriptional activator for some genes and a transcriptional silencer for others. Here we report that in Hep3B cells, cotransfection of NF1/L, NF1/Red1, or NF1/X with the ␣ 1B adrenergic receptor (␣ 1B AR) gene middle (P2) promoter increases P2 activity to more or less the same degree, whereas in DDT 1 MF-2 cells cotransfection of NF1/L or NF1/Red1 causes a small but statistically significant decrease in the P2 promoter activity, and NF1/X causes a greater, 70% inhibition. Further experiments using truncated NF1/X mutants indicate that NF1/X contains both positive and negative regulatory domains. The positive domain, located between amino acids 416 and 505, is active in Hep3B cells, whereas the negative domain, located between amino acids 243 and 416, is active in DDT 1 MF-2 cells. These functional domains are also capable of regulating transcription when isolated from their natural context and fused into the GAL4 binding domain. Furthermore, NF1 affinity purified from rat liver nuclear extracts copurified with a non-DNA binding protein, which can bind to the P2 promoter of the ␣ 1B AR gene via interacting with NF1. Taken together, these findings indicate that NF1/X contains both activation and suppression domains that may be recognized and modulated by cell type-specific cofactors. This may be one of the mechanisms whereby NF1 can activate or suppress the expression of different genes, and it may also underlie the tissue-specific regulation of the ␣ 1B AR gene.The ␣ 1B adrenergic receptor (␣ 1B AR) is a G-protein-coupled receptor that plays an important role in the acute control of cardiovascular homeostasis and metabolic processes in the liver and is also involved in promoting cell proliferation in various tissues (1). Expression of the ␣ 1B AR gene is regulated by hormonal and developmental factors in a tissue-specific manner, as exemplified in hypothyroidism, which increases the level of ␣ 1B AR mRNA in the rat heart but decreases it in the rat liver (2). In primary cultures of rat hepatocytes, high cell density prevents the decline in ␣ 1B AR expression observed at low cell densities (3), whereas in primary cultures of myocardiocytes, increasing cell density decreases ␣ 1B AR expression (4). As a first step toward understanding the molecular mechanisms responsible for such complex regulation, we cloned the rat ␣ 1B AR gene and identified the multiple promoters and cis-acting elements in its regulatory domain (5-7). In subsequent experiments we have found that the dominant P2 promoter interacts with multiple transcription factors including NF1, 1 CP1, AP2, and CREB (8 -10). Further data showed that NF1 and Sp1 are the major transcription factors involved in controlling the P2 promoter in liver and in DDT 1 MF-2 smooth muscle cells, respectively (9).NF1 represents a family of sequence-specific DNA binding proteins that bind to the TGGN 7 CCA consensus sequence (11). NF1 has been reported to act as a transcriptional silencer for some genes, such as the genes e...

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“…These genes lack any predicted perfect NFI dyad symmetric binding sites. While some mammalian promoters have been shown to contain functional hemi NFI binding sites (a single TTGGC or GCCAA site alone) (Cereghini et al, 1987;BoisJoyeux and Danan, 1994;Alonso et al, 1996;Gao et al, 1996), the absence of high-affinity dyad symmetric NFI binding sites within the myosin and exp-2 genes raises the possibility that they may not be direct targets of NFI.…”

Section: Fig 2 Amentioning

confidence: 99%

Lifespan extension and increased pumping rate accompany pharyngeal muscle‐specific expression of nfi‐1 in C. elegans

Lazakovitch

Kalb

Gronostajski

2008

Developmental Dynamics

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Caenorhabditis elegans nfi-1 belongs to the Nuclear Factor I (NFI) family of transcription factors known to regulate metazoan gene expression and development. We showed previously that loss of nfi-1 in worms results in multiple behavioral defects; slower pharyngeal pumping rate, impaired egg laying, defective motility, and a shortened life span. Here, we generated cell-type specific transgenic worms to determine the cells in which nfi-1 must be expressed to rescue the pharyngeal pumping defect. Expression of nfi-1 from the pharyngeal muscle-specific myo-2 promoter, but not from the F25B3.3 or myo-3 promoters, rescued the pharyngeal pumping defect of nfi-1 worms. Surprisingly, myo-2-driven nfi-1 expression also rescued the shortened lifespan of nfi-1 worms, demonstrating a possible cell-autonomous role of nfi-1 in pharyngeal muscle for both phenotypes. We propose some relationships between the pharyngeal pumping and lifespan phenotypes and potential mechanisms of nfi-1 function.

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Transcriptional Regulation of α_1b Adrenergic Receptors (α_1bAR) by Nuclear Factor 1 (NF1): a Decline in the Concentration of NF1 Correlates with the Downregulation of α_1bAR Gene Expression in Regenerating Liver

Cited by 50 publications

References 56 publications

Conjugated bile acids promote ERK1/2 and AKT activation via a pertussis toxin-sensitive mechanism in murine and human hepatocytes

Conjugated bile acids promote ERK1/2 and AKT activation via a pertussis toxin-sensitive mechanism in murine and human hepatocytes

Cell type-specific Transcriptional Activation and Suppression of the α1B Adrenergic Receptor Gene Middle Promoter by Nuclear Factor 1

Lifespan extension and increased pumping rate accompany pharyngeal muscle‐specific expression of nfi‐1 in C. elegans

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