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Query: UNIPROT:Q02556 (
DNA-binding domain
)
6,431
document(s) hit in 31,850,051 MEDLINE articles (0.00 seconds)
SHP
(
short heterodimer partner
) is an unusual orphan receptor that lacks a conventional
DNA-binding domain
. Previous results have shown that it interacts with several other nuclear hormone receptors, including the retinoid and thyroid hormone receptors, and inhibits their ligand-dependent transcriptional activation. Here we show that
SHP
also interacts with estrogen receptors and inhibits their function. In mammalian and yeast two-hybrid systems as well as glutathione-S-transferase pull-down assays,
SHP
interacts specifically with estrogen receptor-alpha (ERalpha) in an agonist-dependent manner. The same assay systems using various deletion mutants of
SHP
map the interaction domain with ERalpha to the same
SHP
sequences required for interaction with the nonsteroid hormone receptors such as retinoid X receptor and thyroid hormone receptor. In transient cotransfection assays,
SHP
inhibits estradiol -dependent activation by ERalpha by about 5-fold. In contrast,
SHP
interacts with ERbeta independent of ligand and reduces its ability to activate transcription by only 50%. These data suggest that
SHP
functions to regulate estrogen signaling through a direct interaction with ERalpha.
...
PMID:Inhibition of estrogen receptor action by the orphan receptor SHP (short heterodimer partner). 977 78
SHP
(
short heterodimer partner
) is an unusual orphan nuclear receptor that contains a putative ligand-binding domain but lacks a conserved
DNA-binding domain
. Although no conventional receptor function has yet been identified,
SHP
has been proposed to act as a negative regulator of nuclear receptor signaling pathways, because it interacts with and inhibits DNA binding and transcriptional activity of various nonsteroid receptors, including thyroid hormone and retinoid receptors. We show here that
SHP
interacts directly with agonist-bound estrogen receptors, ERalpha and ERbeta, and inhibits ER-mediated transcriptional activation.
SHP
specifically targets the ligand-regulated activation domain AF-2 and competes for binding of coactivators such as TIF2. Thus,
SHP
may represent a new category of negative coregulators for ligand-activated nuclear receptors.
SHP
mRNA is widely expressed in rat tissues including certain estrogen target tissues, and subcellular localization studies demonstrate that
SHP
is a nuclear protein, suggesting a biological significance of the
SHP
interactions with ERs. Taken together, these results identify ERs as novel
SHP
targets and suggest that competition for coactivator-binding is a novel mechanism by which
SHP
may inhibit nuclear receptor activation.
...
PMID:The orphan nuclear receptor SHP inhibits agonist-dependent transcriptional activity of estrogen receptors ERalpha and ERbeta. 986 49
Bile acids repress the transcription of cytochrome P450 7A1 (CYP7A1), which catalyzes the rate-limiting step in bile acid biosynthesis. Although bile acids activate the farnesoid X receptor (FXR), the mechanism underlying bile acid-mediated repression of CYP7A1 remained unclear. We have used a potent, nonsteroidal FXR ligand to show that FXR induces expression of
small heterodimer partner
1 (SHP-1), an atypical member of the nuclear receptor family that lacks a
DNA-binding domain
. SHP-1 represses expression of CYP7A1 by inhibiting the activity of liver receptor homolog 1 (LRH-1), an orphan nuclear receptor that is known to regulate CYP7A1 expression positively. This bile acid-activated regulatory cascade provides a molecular basis for the coordinate suppression of CYP7A1 and other genes involved in bile acid biosynthesis.
...
PMID:A regulatory cascade of the nuclear receptors FXR, SHP-1, and LRH-1 represses bile acid biosynthesis. 1103 Mar 32
SHP
(NROB2) is an atypical orphan nuclear receptor that lacks a
DNA-binding domain
but contains a putative ligand-binding domain. Previous studies have revealed that
SHP
interacts with a variety of nuclear receptors and inhibits their transcriptional activity, thereby acting as a corepressor. In this report we identify the glucocorticoid receptor (GR) as a novel downstream target receptor for
SHP
inhibition.
SHP
potently inhibits dexamethasone-induced transcriptional GR activity in mammalian cells, and the inhibition involves a functional second NR-box within
SHP
. Interestingly, this motif shows a high homology with the NR-box in the glucocorticoid and cAMP-inducible GR coactivator PGC-1, indicating similar binding specificity and shared target receptors. We show that
SHP
antagonizes PGC-1 coactivation and, in addition, we identify the PGC- 1-regulated phospho(enol)pyruvate carboxykinase (PEPCK) promoter as a novel target promoter for
SHP
inhibition. This implies a physiologically relevant role for
SHP
in modulating hepatic glucocorticoid action. Furthermore, when coexpressing green fluorescent protein-tagged GR together with
SHP
, an intranuclear redistribution of GR was observed. As inhibition-deficient
SHP
mutants were unable to induce this redistribution, intranuclear tethering of target receptors may represent yet another, previously uncovered, aspect of
SHP
inhibition.
...
PMID:Glucocorticoid signaling is perturbed by the atypical orphan receptor and corepressor SHP. 1232 53
SHP
(
small heterodimer partner
, NR1I0) is an atypical orphan member of the nuclear receptor subfamily in that it lacks a
DNA-binding domain
. It is mostly expressed in the liver, where it binds to and inhibits the function of nuclear receptors.
SHP
is up-regulated by primary bile acids, through the activation of their receptor farnesoid X receptor, leading to the repression of cholesterol 7alpha-hydroxylase (CYP7alpha) expression, the rate-limiting enzyme in bile acid production from cholesterol. PXR (pregnane X receptor, NR1I2) is a broad-specificity sensor that recognizes a wide variety of synthetic drugs as well as endogenous compounds such as bile acid precursors. Upon activation, PXR induces CYP3A and inhibits CYP7alpha, suggesting that PXR can act on both bile acid synthesis and elimination. Indeed, CYP7alpha and CYP3A are involved in biochemical pathways leading to cholesterol conversion into primary bile acids, whereas CYP3A is also involved in the detoxification of toxic secondary bile acid derivatives. Here, we show that PXR is a target for
SHP
. Using pull-down assays, we show that
SHP
interacts with both murine and human PXR in a ligand-dependent manner. From transient transfection assays,
SHP
is shown to be a potent repressor of PXR transactivation. Furthermore, we report that chenodeoxycholic acid and cholic acid, two farnesoid X receptor ligands, induce up-regulation of
SHP
and provoke a repression of PXR-mediated CYP3A induction in human hepatocytes as well as in vivo in mice. These results reveal an elaborate regulatory cascade, tightly controlled by
SHP
, for both the maintenance of bile acid production and detoxification in the liver.
...
PMID:The small heterodimer partner interacts with the pregnane X receptor and represses its transcriptional activity. 1280 10
The orphan nuclear receptor
small heterodimer partner
(
SHP
;
NR0B2
) is an unusual orphan nuclear receptor that lacks a conventional
DNA-binding domain
and acts as a modulator of transcriptional activities of a number of nuclear receptors. We have previously reported that the orphan nuclear receptor ERRgamma activates the
SHP
promoter. In this study, we have found that basic helix-loop-helix (bHLH) transcription factors, the E2A proteins (E47, E12 and E2/5), activated the human but not the mouse
SHP
promoter. In contrast, the tissue-specific E47 heterodimer partner BETA2 repressed the E47- mediated transactivation of the human
SHP
(hSHP) promoter. Using serial deletions and E-box mutant constructs of the hSHP promoter, we identified two E-boxes (E6 and E7) as E47-responsive E-boxes, which are not conserved in the mouse
SHP
promoter. Moreover, gel shift, chromatin immunoprecipitation (ChIP) and northern blot assays demonstrated that E47 directly binds to the hSHP promoter in vivo and in vitro and that Id proteins inhibited E47 binding to the hSHP promoter. Finally, we found that E47 and steroidogenic factor 1 (SF-1), a regulator of the
SHP
promoter, synergistically activate the human but not the mouse
SHP
promoter. Our findings suggest that the E2A proteins differentially regulate the human and mouse
SHP
promoters and cooperate with orphan nuclear receptor SF-1 for transcriptional activation of the hSHP promoter.
...
PMID:Synergistic activation of the human orphan nuclear receptor SHP gene promoter by basic helix-loop-helix protein E2A and orphan nuclear receptor SF-1. 1462 19
Bile acids function as transcriptional regulators for the genes important in bile acid synthesis and cholesterol homeostasis. In this study, we identified angiotensinogen (ANG), the precursor of vasoactive octapeptide angiotensin II, as a novel target gene of bile acids. In human ANG transgenic mice, administration of cholic acid resulted in the down-regulation of human ANG gene expression in the liver. ANG gene expression in HepG2 cells was also repressed by chenodeoxycholic acid. Because the expression of
small heterodimer partner
(
SHP
) mRNA was induced by chenodeoxycholic acid in HepG2 cells, we analyzed the effects of
SHP
on the human ANG promoter. Promoter mutation analysis demonstrated that
SHP
repressed human ANG promoter activity through the element, which has been previously determined as a binding site for hepatocyte nuclear factor-4 (HNF-4).
SHP
repressed human ANG promoter activity only when the HNF-4 expression vector was cotransfected in HeLa cells. Furthermore, we found that
SHP
bound to the HNF-4 N-terminal region including the
DNA-binding domain
and activation function-1 and that
SHP
prevented HNF-4 from binding to the human ANG promoter. These results suggest that bile acids negatively regulate the human ANG gene through the inhibitory effect of
SHP
on HNF-4.
...
PMID:Inhibitory effect of the small heterodimer partner on hepatocyte nuclear factor-4 mediates bile acid-induced repression of the human angiotensinogen gene. 1467 53
Small heterodimer partner
(
SHP
;
NR0B2
) is an unusual orphan nuclear receptor that lacks a conventional
DNA-binding domain
and acts as a modulator of transcriptional activities of a number of nuclear receptors. Herein, we report that the human
SHP
promoter (hSHP) is activated by sterol regulatory element-binding protein-1 (SREBP-1), which regulates the expression of various genes involved in cholesterol and fatty acid synthesis. Overexpression of SREBP-1 activated the human but not mouse
SHP
promoter, although SREBP-2 had little effect on the
SHP
promoter in CV-1 cells. Serial deletion reporter assays revealed that SREBP-1-responsive region is located within the sequences from -243 to -120 bp in the hSHP promoter. DNase I footprinting, gel shift assays, and chromatin immunoprecipitation assays demonstrated that SREBP-1 binds directly to the hSHP promoter. Site-directed mutagenesis made it clear that the hSHP promoter activation by SREBP-1 is mostly mediated by the SRE1 (-186 to -195 bp) in the hSHP promoter, which is not conserved in the mouse
SHP
promoter. Moreover, adenovirus-mediated overexpression of SREBP-1c/ADD-1 induced
SHP
mRNA expression and repressed CYP7A1 expression in HepG2 cells. Finally, we found that a four-nucleotide deletion (-195CT-GAdel) in the hSHP promoter, which is reported to be associated with altered body weight and insulin secretion in human, coincides with the SRE1. This mutation strongly decreased both basal and SREBP-1 dependent activities of the hSHP promoter, because of the reduced binding of SREBP-1 to the mutated SRE1. Overall, our results demonstrate a differential regulation of human and mouse
SHP
promoters by SREBP-1. We propose a possible role of SREBP-1 in the species differential regulation of cholesterol and bile acid homeostasis via a novel mechanism of up-regulation of the hSHP gene expression.
...
PMID:Differential regulation of human and mouse orphan nuclear receptor small heterodimer partner promoter by sterol regulatory element binding protein-1. 1512 50
The nuclear bile acid receptor FXR (farnesoid X receptor) is one of the key factors that suppress bile acid biosynthesis in the liver. PGC-1alpha [PPARgamma (peroxisome-proliferator-activated receptor gamma) co-activator-1alpha] is known to control energy homoeostasis in adipose tissue, skeletal muscle and liver. We performed cell-based reporter assays using the expression system of a GAL4-FXR chimaera, the ligand-binding domain of FXR fused to the
DNA-binding domain
of yeast GAL4, to find the co-activators for FXR. We found that the transcriptional activation of a reporter plasmid by a GAL4-FXR chimaera was strongly enhanced by PGC-1alpha, in a ligand-dependent manner. Transcriptional activation of the
SHP
(
small heterodimer partner
) gene by the FXR-RXRalpha (retinoid X receptor alpha) heterodimer was also enhanced by PGC-1alpha in the presence of CDCA (chenodeoxycholic acid). Co-immunoprecipitation and pull-down studies using glutathione S-transferase-PGC-1alpha fusion proteins revealed that the ligand-binding domain of FXR binds PGC-1alpha in a ligand-influenced manner both in vivo and in vitro. Furthermore, our studies revealed that
SHP
represses its own transcription, and the addition of excess amounts of PGC-1alpha can overcome the inhibitory effect of
SHP
. These observations indicate that PGC-1alpha mediates the ligand-dependent activation of FXR and transcription of
SHP
gene.
...
PMID:The nuclear bile acid receptor FXR is activated by PGC-1alpha in a ligand-dependent manner. 1520 34
Farnesoid X receptor (FXR), the receptor for bile acids, including chenodeoxycholic acid (CDCA), is a member of the nuclear receptor superfamily, which also includes the receptors for retinoic acid, vitamin D (D3), thyroid hormone, thiazolidinedione and 22(R)-hydroxycholesterol. Here, we have evaluated the effects of a series of ligands and their receptors on the promoter activity induced by CDCA/FXR. The kidney cell line, CV1, was cotransfected with FXR-expression plasmid and the luciferase-based reporter gene that has a thymidine kinase promoter fused to the canonical FXR-responsive element or the natural promoter for the
small heterodimer partner
(
SHP
), bile salt export pump (BSEP), and ileum bile acid (I-BABP) gene. D3 and its receptor (VDR) inhibited the transactivation of all four reporter constructs that are enhanced by CDCA/FXR. The effect of D3 on the expression of the BSEP and
SHP
genes in HepG2 cells and that of the I-BABP gene in Caco-2 cells were confirmed by reverse transcription (RT)-PCR. Deletion analysis of VDR revealed that its ligand-binding domain (LBD) is responsible for the repression and the
DNA-binding domain
(
DBD
) is dispensable. Specific interaction between FXR and VDR was detected with the in vitro pull-down assay using chimeric FXR or VDR fused to glutathione-S-transferase.
...
PMID:1,25-dihydroxyvitamin D3 and its receptor inhibit the chenodeoxycholic acid-dependent transactivation by farnesoid X receptor. 1652 42
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