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1. The human orphan nuclear receptor tailless (TLX, NR2E1) is druggable

Author

Fletterick, Robert, Benod, C, Villagomez, R, Filgueira, CS, Hwang, PK, Leonard, PG, Poncet-Montange, G, Rajagopalan, S, Fletterick, RJ, Gustafsson, JA, and Webb, P

Abstract

Nuclear receptors (NRs) are an important group of ligand-dependent transcriptional factors. Presently, no natural or synthetic ligand has been identified for a large group of orphan NRs. Small molecules to target these orphan NRs will provide unique resour

Published
2014

2. Subacute exposure to low concentrations of toluene affects dopamine-mediated locomotor activity in the rat.

Author

von Euler, G, Ogren, SO, Bondy, SC, McKee, M, Warner, M, Gustafsson, JA, Eneroth, P, and Fuxe, K

Subjects
Synaptosomes, Animals, Rats, Inbred Strains, Rats, Calcium, Dopamine, Toluene, Apomorphine, Aldosterone, Corticosterone, Prolactin, Thyrotropin, Receptors, Dopamine, Administration, Inhalation, Injections, Subcutaneous, Motor Activity, Specific Pathogen-Free Organisms, Membrane Fluidity, Male, APOMORPHINE, DOPAMINE RECEPTOR, MEMBRANE FLUIDITY, CALCIUM, PROLACTIN, BASAL GANGLIA, Toxicology, Pharmacology and Pharmaceutical Sciences
Abstract

The effects of low concentrations of toluene (40-80 ppm, 3 days, 6 h/day) were investigated on spontaneous and on apomorphine-induced locomotor activity in the rat, and were correlated to effects on S(-)[N-propyl-3H(N)]-propylnorapomorphine ([3H]NPA) binding in rat neostriatal membranes, on membrane fluidity, membrane leakage, and calcium levels in synaptosomes from the frontoparietal cortex, the neostriatum and the subcortical limbic area, and on serum hormone levels. Toluene exposure (80 ppm, post-exposure delay 18 h) alone did not affect locomotor activity, but attenuated apomorphine-induced (0.05 mg/kg, s.c.) suppression of rearing, and potentiated apomorphine-induced (1 mg/kg, s.c.) increases in locomotion and rearing. Toluene exposure increased the KD value of [3H]NPA binding without affecting the Bmax. All these effects were absent at 40 ppm of toluene or at a post-exposure delay of 42 h. Toluene exposure (80 ppm, post-exposure delay of 18 h) did not affect the serum levels of prolactin, TSH, corticosterone, or aldosterone, or synaptosomal membrane fluidity and calcium levels, whereas membrane leakage was increased in the neostriatum. The present study indicates that the reduction of D-2 receptor affinity by short-term, low-dose toluene exposure is accompanied by a reduced D-2 autoreceptor function and an enhanced postsynaptic D-2 receptor function.

Published
1991

3. Stearoyl-CoA desaturase-1 impairs the reparative properties of macrophages and microglia in the brain

Author

Bogie, JF, Grajchen, E, Wouters, E, Corrales, AG, Dierckx, T, Vanherle, S, Mailleux, J, Gervois, P, Wolfs, E, Dehairs, J, Van Broeckhoven, J, Bowman, AP, Lambrichts, I, Gustafsson, JA, Remaley, AT, Mulder, Monique, Swinnen, JV, Haidar, M, Ellis, SR, Ntambi, JM, Zelcer, N, Hendriks, JJA, Bogie, JF, Grajchen, E, Wouters, E, Corrales, AG, Dierckx, T, Vanherle, S, Mailleux, J, Gervois, P, Wolfs, E, Dehairs, J, Van Broeckhoven, J, Bowman, AP, Lambrichts, I, Gustafsson, JA, Remaley, AT, Mulder, Monique, Swinnen, JV, Haidar, M, Ellis, SR, Ntambi, JM, Zelcer, N, and Hendriks, JJA

Published
2020

4. Identification of a Functional Glucocorticoid Response Element in theCYP3A1/IGC2Gene

Author

Maria Celeste Lechner, Teresa Pereira, Carlstedt-Duke J, and Gustafsson Ja

Subjects
Subfamily, CYP3A, medicine.medical_treatment, Molecular Sequence Data, DNA Footprinting, Biology, Transfection, Mixed Function Oxygenases, Steroid, Receptors, Glucocorticoid, Glucocorticoid receptor, Cytochrome P-450 Enzyme System, Tumor Cells, Cultured, Genetics, medicine, Animals, Cytochrome P-450 CYP3A, Humans, Promoter Regions, Genetic, Glucocorticoids, Molecular Biology, Dexamethasone, Sequence Deletion, Hormone response element, Base Sequence, Cytochrome P450, Cell Biology, General Medicine, Molecular biology, Rats, DNA-Binding Proteins, Gene Expression Regulation, biology.protein, Pregnenolone, medicine.drug
Abstract

The rat CYP3A subfamily of cytochrome P450 consists of steroid- and drug-metabolizing enzymes inducible by pregnenolone 16alpha-carbonitrile and by supra-physiological doses of dexamethasone. The induction of CYP3A by dexamethasone has been proposed to be mediated by a mechanism distinct from the glucocorticoid receptor mediated response. However, a synergistic induction of CYP3A has been observed with physiological doses of glucocorticoids and other CYP3A inducers. We have identified the presence of a glucocorticoid-responsive element in the CYP3A1/IGC2 gene that mediates the induction with physiological doses of glucocorticoids. A 219-bp dexamethasone responsive fragment of the CYP3A1/IGC2 gene localized at -2100/-1882 bp upstream of the transcription initiation site was identified in transfection experiments with HepG2 cells. Maximum induction was achieved with 50-100 nM dexamethasone. DNase I footprinting analysis revealed two glucocorticoid receptor-protected sequences in the 5' flank of the CYP3A1/IGC2 gene. Point mutations in footprint I (-1982/-1960-bp) completely abolished binding and transcription activation whereas a mutation in footprint II (-2001/-1986-bp) only decreased the binding and had no effect on transcription activation. These results led to the conclusion that the glucocorticoid response element present in footprint I mediated the dexamethasone response in transfection experiments with HepG2 cells. Pregnenolone 16alpha-carbonitrile failed to induce any transcriptional effect mediated by this response element in the HepG2 cells.

Published
1998

5. Thermodynamics of sequence-specific glucocorticoid receptor-DNA interactions

Author

Jan Carlstedt-Duke, Johanna Zilliacus, Torleif Haerd, Gustafsson Ja, and Thomas Lundbaeck

Subjects
Hormone response element, Magnetic Resonance Spectroscopy, Base Sequence, Chemistry, Molecular Sequence Data, Thermodynamics, Cooperativity, DNA, Nuclear magnetic resonance spectroscopy, Regulatory Sequences, Nucleic Acid, Biochemistry, Fluorescence spectroscopy, Rats, DNA-Binding Proteins, chemistry.chemical_compound, Receptors, Glucocorticoid, Glucocorticoid receptor, Animals, Humans, Amino Acid Sequence, Binding site, Chemical equilibrium
Abstract

The thermodynamics of sequence-specific DNA-protein interactions provide a complement to structural studies when trying to understand the molecular basis for sequence specificity. We have used fluorescence spectroscopy to study the chemical equilibrium between the wild-type and a triple mutant glucocorticoid receptor DNA-binding domain (GR DBD wt and GR DBDEGA, respectively) and four related DNA-binding sites (response elements). NMR spectroscopy was used to confirm that the structure of the two proteins is very similar in the uncomplexed state. Binding to DNA oligomers containing single half-sites and palindromic binding sites was studied to obtain separate determinations of association constants and cooperativity parameters involved in the dimeric DNA binding. Equilibrium parameters were determined at 10-35 degrees C in 85 mM NaCl, 100 mM KCl, 2 mM MgCl2, and 20 mM Tris-HCl at pH 7.4 (20 degrees C) and at low concentrations of an antioxidant and a nonionic detergent. GR DBDwt binds preferentially to a palindromic consensus glucocorticoid response element (GRE) with an association constant of (7.6 +/- 0.9) x 10(5) M-1 and a cooperativity parameter of 10 +/- 1 at 20 degrees C. GR DBDEGA has the highest affinity for an estrogen response element (ERE) with an association constant of (2.2 +/- 0.3) x 10(5) M-1 and a cooperativity parameter of 121 +/- 17 at 20 degrees C. The difference in cooperativity in the two binding processes, which indicates significant differences in binding modes, was confirmed using gel mobility assays. van't Hoff analysis shows that DNA binding in all cases in entropy driven within the investigated temperature range. We find that delta H0obs and delta S0obs for the formation of a GR DBDwt-GRE versus GR DBDEGA-ERE complex are significantly different despite very similar delta G0obs values. A comparison of GR DBDwt binding to two similar GREs reveals that the discrimination between these two (specific) sites is due to a favorable delta(delta S0obs) which overcompensates an unfavorable delta(delta H0obs), i.e., the sequence specificity is in this case entropy driven. Thus, entropic effects are of decisive importance for the affinity as well as the specificity in GR-DNA interactions. The molecular basis for measured equilibrium and thermodynamic parameters is discussed on the basis of published structures of GR DBD-GRE and ER DBD-ERE complexes.

Published
1994

7. Backbone dynamics of the glucocorticoid receptor DNA-binding domain

Author

Torleif Härd, H. Kovacs, Helena Berglund, Gustafsson Ja, and Karin Dahlman-Wright

Subjects
Binding Sites, Magnetic Resonance Spectroscopy, Protein Conformation, Chemistry, Molecular Sequence Data, Relaxation (NMR), Spin–lattice relaxation, DNA, Nuclear Overhauser effect, DNA-binding domain, Nuclear magnetic resonance spectroscopy, Amides, Biochemistry, Rats, NMR spectra database, Crystallography, Receptors, Glucocorticoid, Protein structure, Nuclear magnetic resonance, Heteronuclear molecule, Escherichia coli, Animals, Amino Acid Sequence, Cloning, Molecular
Abstract

The extent of rapid (picosecond) backbone motions within the glucocorticoid receptor DNA-binding domain (GR DBD) has been investigated using proton-detected heteronuclear NMR spectroscopy on uniformly 15N-labeled protein fragments containing the GR DBD. Sequence-specific 15N resonance assignments, based on two- and three-dimensional heteronuclear NMR spectra, are reported for 65 of 69 backbone amides within the segment C440-A509 of the rat GR in a protein fragment containing a total of 82 residues (MW = 9200). Individual backbone 15N spin-lattice relaxation times (T1), rotating-frame spin-lattice relaxation times (T1 rho), and steady-state (1H)-15N nuclear Overhauser effects (NOEs) have been measured at 11.74 T for a majority of the backbone amide nitrogens within the segment C440-N506. T1 relaxation times and NOEs are interpreted in terms of a generalized order parameter (S2) and an effective correlation time (tau e) characterizing internal motions in each backbone amide using an optimized value for the correlation time for isotropic rotational motions of the protein (tau R = 6.3 ns). Average S2 order parameters are found to be similar (approximately 0.86 +/- 0.07) for various functional domains of the DBD. Qualitative inspection as well as quantitative analysis of the relaxation and NOE data suggests that the picosecond flexibility of the DBD backbone is limited and uniform over the entire protein, with the possible exception of residues S448-H451 of the first zinc domain and a few residues for which relaxation and NOE parameters were not obtained. in particular, we find no evidence for extensive rapid backbone motions within the second zinc domain. Our results therefore suggest that the second zinc domain is not disordered in the uncomplexed state of DBD, although the possibility of slowly exchanging (ordered) conformational states cannot be excluded in the present analysis.

Published
1992

8. Proton NMR studies of the glucocorticoid receptor DNA-binding domain: sequential assignments and identification of secondary structure elements

Author

Jan Carlstedt-Duke, Rolf Boelens, Bonnie A. Maler, Torleif Härd, E. Kellenbach, Gustafsson Ja, Karin Dahlman, Robert Kaptein, Eva I. Hyde, and Leonard P. Freedman

Subjects
Turn (biochemistry), Protein structure, Stereochemistry, Chemistry, Nuclear magnetic resonance spectroscopy, Nuclear Overhauser effect, DNA-binding domain, Biochemistry, Peptide sequence, Protein secondary structure, Peptide Conformation
Abstract

Two protein fragments containing the DNA-binding domain (DBD) of the glucocorticoid receptor (GR) have been studied by two-dimensional 1H NMR spectroscopy. The two peptides (93 and 115 residues, respectively) contain a common segment corresponding to residues C440-I519 of the rat GR or residues C421-I500 of the human GR and include two Zn-binding "finger" domains. The structures of this segment are almost identical in the two protein fragments, as judged from chemical shifts and sequential NOE connectivities. More than 90% of all observable 1H resonances within a 71-residue segment encompassing C440-R510 (rat GR) could be sequentially assigned by standard techniques, and stereospecific assignments could be made for the methyl groups in four valine residues within this segment. Sequential NOE connectivities indicate several elements of secondary structure including two alpha-helical segments consisting of residues S459-E469 and P493-G504, a type I reverse turn between residues R479 and C482, a type II reverse turn between residues L475 and G478, and several regions of extended peptide conformation. No evidence for alpha-helical conformation was found within the two putative zinc-finger domains, indicating that the structures of these domains differ from that of TFIIIA-type zinc fingers. The observation of some very slowly exchanging amide protons in the N-terminal (CI) domain of the DBD in combination with slow rotation of the Y452 aromatic ring indicates that this domain has a restricted conformational flexibility compared to the C-terminal (CII) domain. We also observe several long-range NOE connectivities within C440-R510, suggesting that the sequential assignments presented here will provide a basis for a complete structure determination of this segment of the GR.

Published
1990

9. Cooperativity and specificity in the interactions between DNA and the glucocorticoid receptor DNA binding domain

Author

Jan Carlstedt-Duke, Gustafsson Ja, Karin Dahlman, Torleif Härd, and Rudolf Rigler

Subjects
Hormone response element, Base Sequence, Dimer, Molecular Sequence Data, Fluorescence spectrometry, Cooperative binding, Cooperativity, DNA-binding domain, Biology, Binding, Competitive, Biochemistry, Fluorescence, Potassium Chloride, DNA-Binding Proteins, Kinetics, chemistry.chemical_compound, Receptors, Glucocorticoid, Glucocorticoid receptor, Allosteric Regulation, Models, Chemical, chemistry, Biophysics, Tyrosine, DNA
Abstract

We have employed fluorescence spectroscopy to study the chemical equilibrium between a 115 amino acid protein fragment containing the DNA-binding domain of the human glucocorticoid receptor (DBDr) and a 24-base-pair DNA oligomer containing the glucocorticoid response element (GRE) from the mouse mammary tumor virus promoter region and compared it with the binding to nonspecific DNA at various ionic conditions. We find that binding to both DNAs is cooperative but that DBDr shows a higher affinity for the GRE than for nonspecific DNA and that this difference is more pronounced at increased salt concentrations. Sequence-specific binding to the GRE sequence at 570 mM monovalent cations can be described by a two-site cooperative model, and this supports the notion that DBDr binding to the GRE is enhanced by dimer formation at the recognition site. The product between the (average) association constant for binding to a GRE half-site and the cooperativity parameter was estimated to be K omega = (1-4) x 10(7) M-1 at this salt concentration and 20 degrees C. The sequence-specific binding is not very sensitive to salt concentration in the interval 270-570 mM monovalent cations. However, at lower salt (70 mM) additional binding takes place, presumably nonspecific (cooperative) association to DNA adjacent to the GRE sequence. DBDr binding to nonspecific DNA can be described by the McGhee-von Hippel model for cooperative binding to a chain polymer and is very sensitive to ionic conditions.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1990

10. Myelin-Derived Lipids Modulate Macrophage Activity by Liver X Receptor Activation

Author

Bogie, JFJ, Schalekamp - Timmermans, Sarah, Van, AHT, Irrthum, A, Smeets, HJM, Gustafsson, JA, Steffensen, KR, Mulder, Maarten, Stinissen, P, Hellings, N, Hendriks, JJA, Bogie, JFJ, Schalekamp - Timmermans, Sarah, Van, AHT, Irrthum, A, Smeets, HJM, Gustafsson, JA, Steffensen, KR, Mulder, Maarten, Stinissen, P, Hellings, N, and Hendriks, JJA

Abstract

Multiple sclerosis is a chronic, inflammatory, demyelinating disease of the central nervous system in which macrophages and microglia play a central role. Foamy macrophages and microglia, containing degenerated myelin, are abundantly found in active multiple sclerosis lesions. Recent studies have described an altered macrophage phenotype after myelin internalization. However, it is unclear by which mechanisms myelin affects the phenotype of macrophages and how this phenotype can influence lesion progression. Here we demonstrate, by using genome wide gene expression analysis, that myelin-phagocytosing macrophages have an enhanced expression of genes involved in migration, phagocytosis and inflammation. Interestingly, myelin internalization also induced the expression of genes involved in liver-X-receptor signaling and cholesterol efflux. In vitro validation shows that myelin-phagocytosing macrophages indeed have an increased capacity to dispose intracellular cholesterol. In addition, myelin suppresses the secretion of the pro-inflammatory mediator IL-6 by macrophages, which was mediated by activation of liver-X-receptor beta. Our data show that myelin modulates the phenotype of macrophages by nuclear receptor activation, which may subsequently affect lesion progression in demyelinating diseases such as multiple sclerosis.

Published
2012

11. LXR beta is required for adipocyte growth, glucose homeostasis, and beta cell function

Author

UCL - MD/BICL - Département de biochimie et de biologie cellulaire, Gerin, Isabelle, Dolinsky, VW, Shackman, JG, Kennedy, RT, Chiang, SH, Burant, CF, Steffensen, KR, Gustafsson, JA, MacDougald, OA, UCL - MD/BICL - Département de biochimie et de biologie cellulaire, Gerin, Isabelle, Dolinsky, VW, Shackman, JG, Kennedy, RT, Chiang, SH, Burant, CF, Steffensen, KR, Gustafsson, JA, and MacDougald, OA

Abstract

Liver X receptors (LXR) alpha and beta are nuclear oxysterol receptors with established roles in cholesterol, lipid, and carbohydrate metabolism. Although LXRs have been extensively studied in liver and macrophages, the importance for development and metabolism of other tissues and cell types is not as well characterized. We demonstrate here that although LXR alpha and LXR beta are not required for adipocyte development per se, LXR beta is required for the increase in adipocyte size that normally occurs with aging and diet-induced obesity. Similar food intake and oxygen consumption in LXR beta-/- mice suggests that reduced storage of lipid in adipose tissue is not due to altered energy balance. Despite reduced amounts of adipose tissue, LXR beta-/- mice on a chow diet have insulin sensitivity and levels of adipocyte hormones similar to wild type mice. However, these mice are glucose-intolerant due to impaired glucose-induced insulin secretion. Lipid droplets in pancreatic islets may result from accumulation of cholesterol esters as analysis of islet gene expression reveals that LXR beta is required for expression of the cholesterol transporters, ABCA1 and ABCG1. Our data establish novel roles for LXR beta in adipocyte growth, glucose homeostasis, and beta cell function.

Published
2005

14. Thermodynamics of the glucocorticoid receptor-DNA interaction: binding of wild-type GR DBD to different response elements

Author

Jan Carlstedt-Duke, Gustafsson Ja, Thomas Lundbäck, Torleif Härd, and Carol Cairns

Subjects
Molecular Sequence Data, Thermodynamics, Cooperativity, Biology, Biochemistry, law.invention, chemistry.chemical_compound, Glucocorticoid receptor, Receptors, Glucocorticoid, law, medicine, Binding site, Glucocorticoids, Hormone response element, Binding Sites, Base Sequence, Wild type, Estrogens, DNA, Recombinant Proteins, Spectrometry, Fluorescence, chemistry, Recombinant DNA, Glucocorticoid, medicine.drug
Abstract

We used fluorescence spectroscopy to study the chemical equilibria between an 82-residue protein fragment containing the core conserved region of the glucocorticoid receptor DNA-binding domain (GR DBD) and a palindromic glucocorticoid response element (GRE), a consensus GRE half-site, a consensus estrogen response element (ERE) half-site, and two intermediate half-sites (GRE2 and ERE2). Equilibrium parameters were determined at 20 degrees C and buffer conditions that approximate intracellular conditions. The association constants for GR DBD binding to the GRE (5'TGTTCT3') and GRE2 (5'TGTCCT3') half-sites at 85 mM NaCl, 100 mM KCl, 2 mM MgCl2, and 20 mM Tris-HCl at pH 7.4 and low concentrations of an antioxidant and a nonionic detergent are (1.0 +/- 0.1) x 10(6) M-1 and (5.1 +/- 0.2) x 10(5) M-1, respectively. The association constants for binding to the ERE (5'TGACCT3') and ERE2 (5'TGATCT3') half-sites are < 10(5) M-1. The implications of these numbers for the specificity and affinity for the binding of the intact GR to DNA are discussed. Comparison of GR DBD binding to a GRE half-site and a palindromic GRE sequence allowed us to estimate the cooperativity parameter, omega obs = 25-50, for GR DBD binding to GRE. The thermodynamics of the GR DBD interaction with a GRE half-site were also investigated by determining the temperature dependence of the observed association constant. The nonlinear dependence in ln Kobs as a function of 1/T is consistent with a change in standard heat capacity, delta Cp degree obs = 1.0 +/- 0.2 kcal mol-1 K-1.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1993

15. Dexamethasone reverses glucocorticoid receptor rna depression in multi-drug resistant (MDR) myeloma cell lines

Author

Brönnegard M, Danel-Moore L, and Gustafsson Ja

Subjects
Cancer Research, Drug Resistance, RNA, Pharmacology, Biology, Dexamethasone, Receptors, Glucocorticoid, Glucocorticoid Sensitivity, Glucocorticoid receptor, Oncology, Downregulation and upregulation, Doxorubicin, Cell culture, Tumor Cells, Cultured, medicine, Humans, RNA, Neoplasm, Drug Screening Assays, Antitumor, Multiple Myeloma, Glucocorticoid, medicine.drug
Abstract

Glucocorticoid receptors and glucocorticoid receptor RNA (GR RNA) were measured in doxorubicin resistant myeloma cell lines to investigate the relationship between multi-drug resistance and glucocorticoid sensitivity. Glucocorticoid binding sites and GR RNA were found to be lowered in all the tested doxorubicin resistant cell lines: R10, R40 and R60 compared to the untreated wild type RPMI 8226 cells (Dalton, et al., 1984). The least resistant cell line, R10, maintained a down regulation of GR RNA after 48 hours of dexamethasone (10(-6) M) treatment of the cells. Interestingly, the R10 cell line has been reported to be very sensitive to dexamethasone treatment. However, the GR RNA levels increased in presence of dexamethasone in the most resistant cell line, R40, R60 by comparison to the wild type. Thus, the reduction of GR RNA by doxorubicin treatment appears to be overcome by dexamethasone in the most resistant cell lines. Steroids may be helpful in reversing resistance and maintaining drug sensitive human tumor populations that will continue to respond to cancer chemotherapeutic agents.

Published
1992

25. Estrogen receptor specificity for the effects of estrogen in ovariectomized mice

Author

Lindberg, MK, primary, Weihua, Z, additional, Andersson, N, additional, Moverare, S, additional, Gao, H, additional, Vidal, O, additional, Erlandsson, M, additional, Windahl, S, additional, Andersson, G, additional, Lubahn, DB, additional, Carlsten, H, additional, Dahlman-Wright, K, additional, Gustafsson, JA, additional, and Ohlsson, C, additional

Published
2002
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34. Liver X receptors as regulators of metabolism

Author

Korach-André Marion and Gustafsson Jan-Åke

Subjects
cholesterol, nuclear receptor, oxysterol, transcription, Biology (General), QH301-705.5
Abstract

The liver X receptors (LXR) are crucial regulators of metabolism. After ligand binding, they regulate gene transcription and thereby mediate changes in metabolic pathways. Modulation of LXR and their downstream targets has appeared to be a promising treatment for metabolic diseases especially atherosclerosis and cholesterol metabolism. However, the complexity of LXR action in various metabolic tissues and the liver side effect of LXR activation have slowed down the interest for LXR drugs. In this review, we summarized the role of LXR in the main metabolically active tissues with a special focus on obesity and associated diseases in mammals. We will also discuss the dual interplay between the two LXR isoforms suggesting that they may collaborate to establish a fine and efficient system for the maintenance of metabolism homeostasis.

Published
2015
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37. Effects of subacute treatment with toluene on cerebrocortical alpha- and beta-adrenergic receptors in the rat. Evidence for an increased number and a reduced affinity of beta-adrenergic receptors

Author

Fuxe, K, Martire, Maria, Von Euler, G, Agnati, Lf, Hansson, T, Andersson, K, Gustafsson, Ja, Härfstrand, A., Martire, Maria (ORCID:0000-0003-1650-349X), Fuxe, K, Martire, Maria, Von Euler, G, Agnati, Lf, Hansson, T, Andersson, K, Gustafsson, Ja, Härfstrand, A., and Martire, Maria (ORCID:0000-0003-1650-349X)

Abstract

Subacute treatment with toluene (80-1500 p.p.m.) produces a dose-dependent reduction of affinity and increase in density of the beta-adrenergic antagonist [3H]dihydroalprenolol binding sites in the frontoparietal cortex of the male rat, while the binding characteristics of alpha 1-adrenergic ([3H]WB 4101) and alpha 2-adrenergic ([3H]p-aminoclonidine) binding sites in the same region is unaffected by this treatment as evaluated in vitro. Therefore, it is suggested that the cortical beta-adrenergic receptors are particularly vulnerable to the action of toluene in vivo. It is speculated that as a result cortical beta-adrenergic neurotransmission may be altered following exposure to low concentrations of toluene, possibly related to the physico-chemical properties of toluene, leading to changes in membrane fluidity.

Published
1987

39. Different thresholds of tissue-specific dose-responses to growth hormone in short prepubertal children

Author

Decker Ralph, Nygren Anders, Kriström Berit, Nierop Andreas FM, Gustafsson Jan, Albertsson-Wikland Kerstin, and Dahlgren Jovanna

Subjects
GH deficiency, GH sensitivity, GH responsiveness, Idiopathic short stature, GH dose-effect, Metabolic effects, Lipolysis, Diseases of the endocrine glands. Clinical endocrinology, RC648-665
Abstract

Abstract Background In addition to stimulating linear growth in children, growth hormone (GH) influences metabolism and body composition. These effects should be considered when individualizing GH treatment as dose-dependent changes in metabolic markers have been reported. Hypothesis: There are different dose-dependent thresholds for metabolic effects in response to GH treatment. Method A randomized, prospective, multicentre trial TRN 98-0198-003 was performed for a 2-year catch-up growth period, with two treatment regimens (a) individualized GH dose including six different dose groups ranging from 17–100 μg/kg/day (n=87) and (b) fixed GH dose of 43 μg/kg/day (n=41). The individualized GH dose group was used for finding dose–response effects, where the effective GH dose (ED 50%) required to achieve 50% Δ effect was calculated with piecewise linear regressions. Results Different thresholds for the GH dose were found for the metabolic effects. The GH dose to achieve half of a given effect (ED 50%, with 90% confidence interval) was calculated as 33(±24.4) μg/kg/day for Δ left ventricular diastolic diameter (cm), 39(±24.5) μg/kg/day for Δ alkaline phosphatase (μkat/L), 47(±43.5) μg/kg/day for Δ lean soft tissue (SDS), 48(±35.7) μg/kg/day for Δ insulin (mU/L), 51(±47.6) μg/kg/day for Δ height (SDS), and 57(±52.7) μg/kg/day for Δ insulin-like growth factor I (IGF-I) SDS. Even though lipolysis was seen in all subjects, there was no dose–response effect for Δ fat mass (SDS) or Δ leptin ng/ml in the dose range studied. None of the metabolic effects presented here were related to the dose selection procedure in the trial. Conclusions Dose-dependent thresholds were observed for different GH effects, with cardiac tissue being the most responsive and level of IGF-I the least responsive. The level of insulin was more responsive than that of IGF-I, with the threshold effect for height in the interval between.

Published
2012
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40. Effects of two common polymorphisms in the 3' untranslated regions of estrogen receptor β on mRNA stability and translatability

Author

Gustafsson Jan-Åke, Zhao Chunyan, Putnik Milica, and Dahlman-Wright Karin

Subjects
Genetics, QH426-470
Abstract

Abstract Background The present study represents the first attempt to functionally characterize two common single nucleotide polymorphisms (SNPs) in the 3'untranslated regions (3'UTRs) of estrogen receptor β (ERβ), focusing on the differences between alleles with regard to mRNA stability and translatability. These two ERβ SNPs have been investigated for association with disease in a large number of reports. Results Here we examined allelic expression in breast tumor samples from heterozygous individuals. A significant difference in mRNA levels of the two alleles was observed for one of the SNPs. A cell model system was employed to further investigate potential molecular effects of the two SNPs. We used a modified plasmid, containing the ERβ promoter and ERβ 3'UTRs which include the different alleles of investigated SNPs. Quantitative Real-Time PCR was used to determine mRNA levels after inhibition of transcription by actinomycin D, and a luciferase assay was used to determine protein levels. The obtained results suggested that there was no difference in mRNA stability or translatability between the alleles of investigated SNPs. Conclusion Our results indicate that observed associations between ERβ 3'UTR SNPs and disease susceptibility are due to linkage disequilibrium with another gene variant, rather than the variant itself being the susceptibility factor.

Published
2009
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41. Functional and genetic analysis in type 2 diabetes of Liver X receptor alleles – a cohort study

Author

Gustafsson Jan-Åke, Brismar Kerstin, Östenson Claes G, Efendic Suad, Lecoeur Cecile, Gu Harvest F, Nilsson Maria, Dahlman Ingrid, Froguel Philippe, Vaxillaire Martine, Dahlman-Wright Karin, and Steffensen Knut R

Subjects
Internal medicine, RC31-1245, Genetics, QH426-470
Abstract

Abstract Background Liver X receptor alpha (LXRA) and beta (LXRB) regulate glucose and lipid homeostasis in model systems but their importance in human physiology is poorly understood. This project aimed to determine whether common genetic variations in LXRA and LXRB associate with type 2 diabetes (T2D) and quantitative measures of glucose homeostasis, and, if so, reveal the underlying mechanisms. Methods Eight common single nucleotide polymorphisms in LXRA and LXRB were analyzed for association with T2D in one French cohort (N = 988 cases and 941 controls), and for association with quantitative measures reflecting glucose homeostasis in two non-diabetic population-based samples comprising N = 697 and N = 1344 adults. Investigated quantitative phenotypes included fasting plasma glucose, serum insulin, and HOMAIR as measure of overall insulin resistance. An oral glucose tolerance test was performed in N = 1344 of adults. The two alleles of the proximal LXRB promoter, differing only at the SNP rs17373080, were cloned into reporter vectors and transiently transfected, whereupon allele-specific luciferase activity was measured. rs17373080 overlapped, according to in silico analysis, with a binding site for Nuclear factor 1 (NF1). Promoter alleles were tested for interaction with NF1 using direct DNA binding and transactivation assays. Results Genotypes at two LXRB promoter SNPs, rs35463555 and rs17373080, associated nominally with T2D (P values 0.047 and 0.026). No LXRA or LXRB SNP associated with quantitative measures reflecting glucose homeostasis. The rs17373080 C allele displayed higher basal transcription activity (P value < 0.05). The DNA-mobility shift assay indicated that oligonucleotides corresponding to either rs17373080 allele bound NF1 transcription factors in whole cell extracts to the same extent. Different NF1 family members showed different capacity to transactivate the LXRB gene promoter, but there was no difference between promoter alleles in NF1 induced transactivation activity. Conclusion Variations in the LXRB gene promoter may be part of the aetiology of T2D. However, the association between LXRB rs35463555 and rs17373080, and T2D are preliminary and needs to be investigated in additional larger cohorts. Common genetic variation in LXRA is unlikely to affect the risk of developing T2D or quantitative phenotypes related to glucose homeostasis.

Published
2009
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42. Impact of estrogen receptor gene polymorphisms and mRNA levels on obesity and lipolysis – a cohort study

Author

Arner Peter, Gustafsson Jan-Åke, Jiao Hong, Dahlman Ingrid, Nilsson Maria, and Dahlman-Wright Karin

Subjects
Internal medicine, RC31-1245, Genetics, QH426-470
Abstract

Abstract Background The estrogen receptors α and β (ESR1, ESR2) have been implicated in adiposity, lipid metabolism and feeding behaviour. In this report we analyse ESR1 and ESR2 gene single nucleotide polymorphisms (SNPs) for association with obesity. We also relate adipose tissue ESR1 mRNA levels and ESR1 SNPs to adipocyte lipolysis and lipogenesis phenotypes. Methods 23 ESR1 and 11 ESR2 tag-SNPs, covering most of the common haplotype variation in each gene according to HAPMAP data, were analysed by Chi2 for association with obesity in a cohort comprising 705 adults with severe obesity and 402 lean individuals. Results were replicated in a cohort comprising 837 obese and 613 lean subjects. About 80% of both cohorts comprised women and 20% men. Adipose tissue ESR1 mRNA was quantified in 122 women and related to lipolysis and lipogenesis by multiple regression. ESR1 SNPs were analysed for association with adipocyte lipolysis and lipogenesis phenotypes in 204 obese women by simple regression. Results No ESR1 SNP was associated with obesity. Five ESR2 SNPs displayed nominal significant allelic association with obesity in women and one in men. The two ESR2 SNPs associated with obesity with nominal P value < 0.01 were genotyped in a second cohort where no association with obesity was observed. There was an inverse correlation between ESR1 mRNA levels in abdominal subcutaneous (sc) adipose tissue and basal lipolysis, as well as responsiveness to adrenoceptor agonists independent of age and BMI (P value 0.009–0.045). ESR1 rs532010 was associated with lipolytic sensitivity to noradrenaline (nominal P value 0.012), and ESR1 rs1884051 with responsiveness to the non-selective beta-adrenoceptor agonist isoprenaline (nominal P value 0.05). These associations became non-significant after Bonferroni correction. Conclusion ESR1 gene alleles are unlikely to be a major cause of obesity in women. A minor importance of ESR2 on severe obesity cannot be excluded. The inverse correlation between ESR1 mRNA levels and lipolytic responsiveness to adrenoceptor agonists implies that low adipose tissue ESR1 levels attenuate catecholamine resistance in sc fat cells of obese women hereby contributing to loss of sc and gain of visceral fat. There is no evidence for a genetic impact of ESR1 on lipolysis or lipogenesis.

Published
2007
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43. Estren promotes androgen phenotypes in primary lymphoid organs and submandibular glands

Author

Gustafsson Jan-Åke, Lindberg Marie, Skrtic Sofia, Jochems Caroline, Erlandsson Malin C, Hasséus Bengt, Islander Ulrika, Ohlsson Claes, and Carlsten Hans

Subjects
Immunologic diseases. Allergy, RC581-607
Abstract

Abstract Background Estrogens and androgens have extensive effects on the immune system, for example they suppress both T and B lymphopoiesis in thymus and bone marrow. Submandibular glands are sexually dimorphic in rodents, resulting in larger granular convoluted tubules in males compared to females. The aim of the present experiments was to investigate the estrogenic and androgenic effects of 4-estren-3α,17β-diol (estren) on thymus, bone marrow and submandibular glands, and compare the effects to those of 17β-estradiol (E2) and 5α-dihydrotestosterone (DHT), respectively. Estrogen receptors (ERs) were blocked by treatment of mice with the ER-antagonist ICI 182,780; also, knock-out mice lacking one or both ERs were used. Results As expected, the presence of functional ERs was mandatory for all the effects of E2. Similar to DHT-treatment, estren-treatment resulted in decreased thymus weight, as well as decreased frequency of bone marrow B cells. Treatment with estren or DHT also resulted in a shift in submandibular glands towards an androgen phenotype. All the effects of estren and DHT were independent of ERs. Conclusion Our study is the first to show that estren has similar effects as the androgen DHT on lymphopoiesis in thymus and bone marrow, and on submandibular glands, and that these effects are independent of estrogen receptors. This supports the hypothesis of estren being able to signal through the androgen receptor.

Published
2005
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44. The oxysterol-CXCR2 axis plays a key role in the recruitment of tumor-promoting neutrophils

Author

Claudia Lanterna, Vincenzo Russo, Eduardo J. Villablanca, Ivano Eberini, Alessandro Prinetti, Silvano Sozzani, Laura Raccosta, Elena Chiricozzi, Claudia Martini, Maria Letizia Trincavelli, Cristina Sensi, Andrea Musumeci, Safiyè Gonzalvo Feo, Andrea Leiva, Claudio Doglioni, Daniela Maggioni, Sandro Sonnino, Laura Mauri, Jan-Åke Gustafsson, Catia Traversari, Simona Daniele, Aida Paniccia, Raffaella Fontana, J. Rodrigo Mora, Knut R. Steffensen, Maria Grazia Ciampa, Claudio Bordignon, Raccosta, L, Fontana, R, Maggioni, D, Lanterna, C, Villablanca, Ej, Paniccia, A, Musumeci, A, Chiricozzi, E, Trincavelli, Ml, Daniele, S, Martini, C, Gustafsson, Ja, Doglioni, Claudio, Feo, Sg, Leiva, A, Ciampa, Mg, Mauri, L, Sensi, C, Prinetti, A, Eberini, I, Mora, Jr, Bordignon, Claudio, Steffensen, Kr, Sonnino, S, Sozzani, S, Traversari, C, and Russo, V.

Subjects
Oxysterol, Neutrophils, Immunology, Biology, Ligands, Mass Spectrometry, Receptors, Interleukin-8B, Article, Receptors, G-Protein-Coupled, Mice, Immune system, Neoplasms, polycyclic compounds, Immunology and Allergy, Animals, Antigens, Ly, Humans, Myeloid Cells, CXC chemokine receptors, Dendritic cell migration, Liver X receptor, Chromatography, High Pressure Liquid, Cell Proliferation, Liver X Receptors, Immunosuppression Therapy, CD11b Antigen, Neovascularization, Pathologic, Cell growth, Chemotaxis, Orphan Nuclear Receptors, Hydroxycholesterols, Cell biology, Disease Models, Animal, Sterols, HEK293 Cells, lipids (amino acids, peptides, and proteins), Signal transduction, Signal Transduction
Abstract

Tumor-derived oxysterols recruit protumor neutrophils in an LXR-independent, CXCR2-dependent manner, thus favoring tumor growth by promoting neoangiogenesis and immunosuppression., Tumor-infiltrating immune cells can be conditioned by molecules released within the microenvironment to thwart antitumor immune responses, thereby facilitating tumor growth. Among immune cells, neutrophils play an important protumorigenic role by favoring neoangiogenesis and/or by suppressing antitumor immune responses. Tumor-derived oxysterols have recently been shown to favor tumor growth by inhibiting dendritic cell migration toward lymphoid organs. We report that tumor-derived oxysterols recruit protumor neutrophils in a liver X receptor (LXR)–independent, CXCR2-dependent manner, thus favoring tumor growth by promoting neoangiogenesis and immunosuppression. We demonstrate that interfering with the oxysterol–CXCR2 axis delays tumor growth and prolongs the overall survival of tumor-bearing mice. These results identify an unanticipated protumor function of the oxysterol–CXCR2 axis and a possible target for cancer therapy.

Published
2013

45. Tumor-mediated liver X receptor-α activation inhibits CC chemokine receptor-7 expression on dendritic cells and dampens antitumor responses

Author

Alessandro Prinetti, Vincenzo Russo, Laura Raccosta, Daniela Maggioni, Raffaella Fontana, Sandro Sonnino, Marco Bregni, Francesca Sanvito, Catia Traversari, Eduardo J. Villablanca, Claudio Bordignon, Claudio Doglioni, Dan Zhou, Barbara Valentinis, Knut R. Steffensen, Aurora Negro, Maurilio Ponzoni, Jan-Åke Gustafsson, Villablanca, Ej, Raccosta, L, Zhou, D, Fontana, R, Maggioni, D, Negro, A, Sanvito, F, Ponzoni, M, Valentinis, B, Bregni, M, Prinetti, A, Steffensen, Kr, Sonnino, S, Gustafsson, Ja, Doglioni, C, Bordignon, C, Traversari, C, and Russo, V

Subjects
Receptors, CCR7, Chemokine receptor CCR5, Immunoglobulins, chemical and pharmacologic phenomena, C-C chemokine receptor type 7, C-C chemokine receptor type 6, General Biochemistry, Genetics and Molecular Biology, Mice, Antigens, CD, Cell Movement, Cell Line, Tumor, Animals, Humans, Liver X receptor, Melanoma, Liver X Receptors, Membrane Glycoproteins, biology, CCL18, Dendritic Cells, Neoplasms, Experimental, General Medicine, Orphan Nuclear Receptors, CCL20, Gene Expression Regulation, Immunology, biology.protein, Cancer research, Tumor Escape, Lymph Nodes, CCL25, CC chemokine receptors, Signal Transduction
Abstract

Sterol metabolism has recently been linked to innate and adaptive immune responses through liver X receptor (LXR) signaling. Whether products of sterol metabolism interfere with antitumor responses is currently unknown. Dendritic cells (DCs) initiate immune responses, including antitumor activity after their CC chemokine receptor-7 (CCR7)-dependent migration to lymphoid organs. Here we report that human and mouse tumors produce LXR ligands that inhibit CCR7 expression on maturing DCs and, therefore, their migration to lymphoid organs. In agreement with this observation, we detected CD83(+)CCR7(-) DCs within human tumors. Mice injected with tumors expressing the LXR ligand-inactivating enzyme sulfotransferase 2B1b (SULT2B1b) successfully controlled tumor growth by regaining DC migration to tumor-draining lymph nodes and by developing overt inflammation within tumors. The control of tumor growth was also observed in chimeric mice transplanted with bone marrow from mice lacking the gene encoding LXR-alpha (Nr1h3(-/-) mice) Thus, we show a new mechanism of tumor immunoescape involving products of cholesterol metabolism. The manipulation of this pathway could restore antitumor immunity in individuals with cancer. Sterol metabolism has recently been linked to innate and adaptive immune responses through liver X receptor (LXR) signaling. Whether products of sterol metabolism interfere with antitumor responses is currently unknown. Dendritic cells (DCs) initiate immune responses, including antitumor activity after their CC chemokine receptor-7 (CCR7)-dependent migration to lymphoid organs. Here we report that human and mouse tumors produce LXR ligands that inhibit CCR7 expression on maturing DCs and, therefore, their migration to lymphoid organs. In agreement with this observation, we detected CD83(+)CCR7(-) DCs within human tumors. Mice injected with tumors expressing the LXR ligand-inactivating enzyme sulfotransferase 2B1b (SULT2B1b) successfully controlled tumor growth by regaining DC migration to tumor-draining lymph nodes and by developing overt inflammation within tumors. The control of tumor growth was also observed in chimeric mice transplanted with bone marrow from mice lacking the gene encoding LXR-alpha (Nr1h3(-/-) mice) Thus, we show a new mechanism of tumor immunoescape involving products of cholesterol metabolism. The manipulation of this pathway could restore antitumor immunity in individuals with cancer.

Published
2010

46. ERdj5, an Endoplasmic Reticulum (ER)-resident Protein Containing DnaJ and Thioredoxin Domains, Is Expressed in Secretory Cells or following ER Stress

Author

Roberto Sitia, Saku Leinonen, Gloria Bertoli, Markku Pelto Huikko, Jan-Åke Gustafsson, Antonio Miranda-Vizuete, Paula Cunnea, Anastasios E. Damdimopoulos, Stefan Hermann, Giannis Spyrou, Thomas Simmen, Cunnea, Pm, MIRANDA VIZUETE, A, Bertoli, G, Simmen, T, Damdimopoulos, Ae, Hermann, S, Leinonen, S, Huikko, Mp, Gustafsson, Ja, Sitia, Roberto, and Spyrou, G.

Subjects
Protein Folding, Molecular chaperones, Carrier proteins, Molecular Sequence Data, Biology, Biochemistry, Chromosomes, Thioredoxins, Transcription (biology), Humans, Amino Acid Sequence, Cloning, Molecular, Thioredoxin, Molecular Biology, Endoplasmic Reticulum Chaperone BiP, Caenorhabditis elegans, Heat-Shock Proteins, Endoplasmic reticulum, Chromosome Mapping, STIM1, Cell Biology, HSP40 Heat-Shock Proteins, biology.organism_classification, Cell biology, Protein Transport, Secretory protein, Unfolded protein response, Protein folding, Sequence Alignment, Adenosine triphosphate, Cloning
Abstract

8 páginas, 7 figuras., A complex array of chaperones and enzymes reside in the endoplasmic reticulum (ER) to assist the folding and assembly of and the disulfide bond formation in nascent secretory proteins. Here we characterize a novel human putative ER co-chaperone (ERdj5) containing domains resembling DnaJ, protein-disulfide isomerase, and thioredoxin domains. Homologs of ERdj5 have been found in Caenorhabditis elegans and Mus musculus. In vitro experiments demonstrated that ERdj5 interacts via its DnaJ domain with BiP in an ATP-dependent manner. ERdj5 is a ubiquitous protein localized in the ER and is particularly abundant in secretory cells. Its transcription is induced during ER stress, suggesting potential roles for ERdj5 in protein folding and translocation across the ER membrane., This work was supported in part by Swedish Medical Research Council Projects 13X-10370 and 19X-11622-03C and by grants from the Medical Research Fund of Tampere University Hospital, the Funds of University of Tampere, the Karolinska Institute, Södertörns Högskola, the Associazione Italiana per la Ricerca sul Cancro (AIRC), the Italian Ministry of University and Research (MIUR, Center of Excellence in Physiopathology of Cell Differentiation), PRIN (2002.058218_006), and Telethon (GP0117/01).

Published
2003

47. Development of a gratitude intervention model and investigation of the effects of such a program on employee well-being, engagement, job satisfaction and psychological capital.

Author

Harty B, Gustafsson JA, Thorén M, Möller A, and Björkdahl A

Abstract

Background: In a demanding working life, it is important to determine how individuals can thrive at work. In a previous study we investigated whether a program of gratitude interventions can increase psychological wellbeing, engagement, job satisfaction, and psychological capital showing promising results., The Objective: of the present study was to present the development of a manager coached group intervention program related to gratitude at workplaces and to investigate the effects of such a program on the same variables., Methods: The intervention included five group sessions of gratitude dialogue between employees, supervised by their first line managers. Participants were assigned to an intervention or control group. Assessments were made before and after the intervention program and followed-up at 6 months post-intervention. Both quantitative and qualitative analyses were performed. Both groups completed instruments measuring positive psychological capital (PCQ), work engagement (UWES), psychological wellbeing (PGWB-S), and job satisfaction (aJDI). All managers were interviewed after the intervention., Result: Compared with the control group the gratitude dialogue intervention was found to significantly enhance psychological wellbeing, engagement, and job satisfaction. The results were supported by the interviews with managers., In Conclusion: our results suggest that gratitude dialogues at work may be an effective way of improving employee wellbeing. Suggestions on how to improve the results from this kind of gratitude intervention further are presented.

Published
2024
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48. Activation of ERβ hijacks the splicing machinery to trigger R-loop formation in triple-negative breast cancer.

Author

Wang D, Tang M, Zhang P, Yang K, Huang L, Wu M, Shen Q, Yue J, Wang W, Gong Y, Warner M, Dai L, He H, Yang Z, Gustafsson JA, and Zhou S

Subjects
Humans, Combined Modality Therapy, MDA-MB-231 Cells, Protein Binding, Binding Sites, Estrogen Receptor beta agonists, Estrogen Receptor beta metabolism, R-Loop Structures, Splicing Factor U2AF chemistry, Splicing Factor U2AF genetics, Splicing Factor U2AF metabolism, Triple Negative Breast Neoplasms drug therapy, Triple Negative Breast Neoplasms genetics, Triple Negative Breast Neoplasms metabolism, Alternative Splicing drug effects, Benzopyrans pharmacology, Benzopyrans therapeutic use
Abstract

Triple-negative breast cancer (TNBC) is a subtype of breast cancer with aggressive behavior and poor prognosis. Current therapeutic options available for TNBC patients are primarily chemotherapy. With our evolving understanding of this disease, novel targeted therapies, including poly ADP-ribose polymerase (PARP) inhibitors, antibody-drug conjugates, and immune-checkpoint inhibitors, have been developed for clinical use. Previous reports have demonstrated the essential role of estrogen receptor β (ERβ) in TNBC, but the detailed molecular mechanisms downstream ERβ activation in TNBC are still far from elucidated. In this study, we demonstrated that a specific ERβ agonist, LY500307, potently induces R-loop formation and DNA damage in TNBC cells. Subsequent interactome experiments indicated that the residues 151 to 165 of U2 small nuclear RNA auxiliary factor 1 (U2AF1) and the Trp 439 and Lys 443 of ERβ were critical for the binding between U2AF1 and ERβ. Combined RNA sequencing and ribosome sequencing analysis demonstrated that U2AF1-regulated downstream RNA splicing of 5-oxoprolinase ( OPLAH ) could affect its enzymatic activity and is essential for ERβ-induced R-loop formation and DNA damage. In clinical samples including 115 patients from The Cancer Genome Atlas (TCGA) and 32 patients from an in-house cohort, we found a close correlation in the expression of ESR2 and U2AF1 in TNBC patients. Collectively, our study has unraveled the molecular mechanisms that explain the therapeutic effects of ERβ activation in TNBC, which provides rationale for ERβ activation-based single or combined therapy for patients with TNBC., Competing Interests: Competing interests statement:The authors declare no competing interest.

Published
2024
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49. Estrogen receptor β attenuates renal fibrosis by suppressing the transcriptional activity of Smad3.

Author

Cao R, Su W, Sheng J, Guo Y, Su J, Zhang C, Wang H, Tang Y, Chen L, Qiao R, Chen X, Huang X, Zhou Y, Zhu L, Bai Z, Zhang X, Gustafsson JA, Wan Q, Lan HY, and Guan Y

Subjects
Animals, Mice, Estrogen Receptor beta genetics, Estrogen Receptor beta metabolism, Fibrosis, Kidney pathology, Transforming Growth Factor beta1 metabolism, Renal Insufficiency, Chronic drug therapy, Ureteral Obstruction genetics, Ureteral Obstruction metabolism
Abstract

Renal fibrosis (RF) is a common pathway leading to chronic kidney disease (CKD), which lacks effective treatment. While estrogen receptor beta (ERβ) is known to be present in the kidney, its role in RF remains unclear. The present study aimed to investigate the role and underlying mechanism of ERβ during RF progression in patients and animal models with CKD. We found that ERβ was highly expressed in the proximal tubular epithelial cells (PTECs) in healthy kidneys but its expression was largely lost in patients with immunoglobin A nephropathy (IgAN) and in mice with unilateral ureter obstruction (UUO) and subtotal nephrectomy (5/6Nx). ERβ deficiency markedly exacerbated, whereas ERβ activation by WAY200070 and DPN attenuated RF in both UUO and 5/6Nx mouse models, suggesting a protective role of ERβ in RF. In addition, ERβ activation inhibited TGF-β1/Smad3 signaling, while loss of renal ERβ was associated with overactivation of the TGF-β1/Smad3 pathway. Furthermore, deletion or pharmacological inhibition of Smad3 prevented the loss of ERβ and RF. Mechanistically, activation of ERβ competitively inhibited the association of Smad3 with the Smad-binding element, thereby downregulating the transcription of the fibrosis-related genes without altering Smad3 phosphorylation in vivo and in vitro. In conclusion, ERβ exerts a renoprotective role in CKD by blocking the Smad3 signaling pathway. Thus, ERβ may represent as a promising therapeutic agent for RF., Competing Interests: Declaration of competing interest The authors declare no disclosures of interests., (Copyright © 2023. Published by Elsevier B.V.)

Published
2023
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50. Liver X receptors and estrogen receptor β, two players in a rare subtype of NSCLC.

Author

Wu W, Sarhadi M, Song X, Xue J, Dai Y, and Gustafsson JA

Subjects
Mice, Animals, Estrogen Receptor beta genetics, Estrogen Receptor beta metabolism, Liver X Receptors genetics, Lung metabolism, Carcinoma, Non-Small-Cell Lung genetics, Carcinoma, Non-Small-Cell Lung metabolism, Lung Neoplasms metabolism
Abstract

Liver X receptors (LXRαβ) play essential roles in the maintenance of the normal functions of macrophages, in modulation of immune system responses and cholesterol homeostasis. We have reported that LXRαβ -/- mice develop squamous cell lung cancer. We now report that those LXRαβ -/- mice, which live to 18-months of age, spontaneously develop a second type of lung cancer resembling a rare subtype of NSCLC (TTF-1 and P63-positive). The lesions are characterized as follows: a high proliferation rate; a marked accumulation of abnormal macrophages; an increase in the number of regulatory T cells; a remarkably low level of CD8 + cytotoxic T lymphocytes; enhanced TGFβ signaling; an increased expression of matrix metalloproteinases accompanied by degradation of lung collagen; and a loss of estrogen receptor β (ERβ). Because NSCLC is associated with cigarette smoking, we investigated the possible links between loss of LXRαβ and CS. A Kaplan-Meier Plotter database revealed reduced expression of LXRαβ and ERβ was correlated with low overall survival (OS). Thus, reduction of LXRαβ expression by cigarette smoking may be one mechanism through which CS causes lung cancer. The possibility that maintenance of LXRαβ and ERβ signaling could be used in the treatment of NSCLC needs further investigation., Competing Interests: Competing Interests: The authors have declared that no competing interest exists., (© The author(s).)

Published
2023
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