Your search keyword '"Ina Nordström"' showing total 9 results

1. Down-regulation of endothelial cell estrogen receptor expression by the inflammation promoter LPS

Author

Kristina E. Andersson, Ina Nordström, Anders Holm, Bengt-Olof Nilsson, and Per Hellstrand

Subjects

Lipopolysaccharides, medicine.medical_specialty, medicine.drug_class, Blotting, Western, Down-Regulation, Estrogen receptor, Biology, Biochemistry, Dexamethasone, Cell Line, Mice, Endocrinology, Downregulation and upregulation, Internal medicine, polycyclic compounds, medicine, Animals, Estrogen Receptor beta, Protein Isoforms, RNA, Messenger, Glucocorticoids, Molecular Biology, Cells, Cultured, Inflammation, Messenger RNA, Reverse Transcriptase Polymerase Chain Reaction, Estrogen Receptor alpha, Endothelial Cells, Molecular biology, Endothelial stem cell, Blot, Gene Expression Regulation, Cell culture, Estrogen, hormones, hormone substitutes, and hormone antagonists, Glucocorticoid, medicine.drug

Abstract

Endothelial cells express both estrogen receptor (ER) alpha and beta. The objective of this study was to investigate if and how mediators of inflammation regulate endothelial cell ERalpha and ERbeta expression. ERalpha and ERbeta transcript and protein expression were determined by real-time quantitative PCR and Western blotting, respectively, in endothelial cell line bEnd.3 cells stimulated with the inflammation promoter lipopolysaccharide (E. coli LPS). Stimulation with LPS (500 ng/ml and 10 microg/ml) for 4 days reduced both ERalpha and ERbeta mRNA levels. The glucocorticoid dexamethasone (1 microM) had no effect on LPS-induced attenuation of ERalpha and beta transcript expression. Full-length 66-67 kDa ERalpha protein was unaffected by 4 days stimulation with LPS, while the 46-kDa ERalpha isoform was reduced by about 20%. ERbeta protein was reduced by about 40% by LPS at 4 days. Treatment with 17beta-estradiol (E(2), 100 nM) for 4 days increased ERbeta mRNA by about 8 times but had no effect on ERalpha mRNA level. The E(2)-induced increase in ERbeta transcript was not associated with increased ERbeta protein. E(2) increased ERbeta mRNA expression also in the presence of LPS, suggesting that inflammation-induced impairment of ERbeta signalling is rescued by estrogen.

Published

2010

2. Injury to rat carotid arteries causes time-dependent changes in gene expression in contralateral uninjured arteries

Author

Francesco Rossi, Francesco Onorati, Pasquale Santè, Attilio Renzulli, Umberto Galderisi, Maurizio Cotrufo, Liberato Berrino, Mauro Finicelli, Antonino Cascino, Per Hellstrand, Cesare Quarto, Marisa De Feo, Ina Nordström, Amalia Forte, Marilena Cipollaro, Pasquale De Luca, Forte, A., Finicelli, M., DE LUCA, P., Nordström, I., Onorati, F., Quarto, C., Sante', Pasquale, Renzulli, A., Galderisi, Umberto, Berrino, Liberato, DE FEO, Marisa, Hellstrand, P., Rossi, Francesco, Cotrufo, M., Cascino, A., and Cipollaro, Marilena

Subjects

Male, Pathology, medicine.medical_specialty, Carotid Artery, Common, medicine.medical_treatment, Blotting, Western, Arteriotomy, rat carotid arterie, Rats, Inbred WKY, Lesion, vascular injury, Restenosis, Renin–angiotensin system, medicine, Animals, remodelling, Oligonucleotide Array Sequence Analysis, Reverse Transcriptase Polymerase Chain Reaction, business.industry, Gene Expression Profiling, General Medicine, Anatomy, Vascular surgery, medicine.disease, Angiotensin II, Rats, medicine.anatomical_structure, Gene Expression Regulation, inflammation, medicine.symptom, Carotid Artery Injuries, business, microarray, Signal Transduction, Blood vessel, Artery

Abstract

Vascular surgery aimed at stenosis removal induces local reactions often leading to restenosis. Although extensive analysis has been focused on pathways activated in injured arteries, little attention has been devoted to associated systemic vascular reactions. The aim of the present study was to analyse changes occurring in contralateral uninjured rat carotid arteries in the acute phase following unilateral injury. WKY (Wistar–Kyoto) rats were subjected to unilateral carotid arteriotomy. Contralateral uninjured carotid arteries were harvested from 4 h to 7 days after injury. Carotid arteries were also harvested from sham-operated rats and uninjured rats. Carotid morphology and morphometry were examined. Affymetrix microarrays were used for differential analysis of gene expression. A subset of data was validated by real-time RT–PCR (reverse transcription–PCR) and verified at the protein level by Western blotting. A total of 1011 genes were differentially regulated in contralateral uninjured carotid arteries from 4 h to 7 days after arteriotomy (P

Published

2008

3. Rat arterial smooth muscle devoid of ryanodine receptor function: effects on cellular Ca2+handling

Author

Karl Dreja, Ina Nordström, and Per Hellstrand

Subjects

Pharmacology, medicine.medical_specialty, Thapsigargin, Ryanodine receptor, Biology, Organ culture, Contractility, chemistry.chemical_compound, Endocrinology, chemistry, Internal medicine, medicine, medicine.symptom, Receptor, Caffeine, Cyclopiazonic acid, Muscle contraction

Abstract

The roles of intracellular Ca2+ stores and ryanodine (Ry) receptors for vascular Ca2+ homeostasis and viability were investigated in rat tail arterial segments kept in organ culture with Ry (10 100 M) for up to 4 days. Acute exposure to Ry or the non-deactivating ryanodine analogue C10-Oeq glycyl ryanodine (10 M) eliminated Ca2+ release responses to caffeine (20 mM) and noradrenaline (NA, 10 M), whereas responses to NA, but not caffeine, gradually returned to normal within 4 days of exposure to Ry. Ry receptor protein was detected on Western blots in arteries cultured either with or without Ry. Brief Ca2+ release events (sparks) were absent after culture with Ry, whereas Ca2+ waves still occurred. The propagation velocity of waves was equal (19 m s-1) in tissue cultured either with or without Ry. Inhibition of Ca2+ accumulation into the sarcoplasmic reticulum (SR) by culture with caffeine (5 mM), cyclopiazonic acid or thapsigargin (both 10 M) decreased contractility due to Ca2+-induced cell damage. In contrast, culture with Ry did not affect contractility. Removal of Ca2+ from the cytosol following a Ca2+ load was retarded after Ry culture. Thapsigargin reduced the rate of Ca2+ removal in control cultured rings, but had no effect after Ry culture. It is concluded that intracellular Ca2+ stores recover during chronic Ry treatment, while Ry receptors remain non-functional. Ry receptor activity is required for Ca2+ sparks and for SR-dependent recovery from a Ca2+ load, but not for Ca2+ waves or basal Ca2+ homeostasis. (Less)

Published

2001

4. Long-term effects of Ca2+on structure and contractility of vascular smooth muscle

Author

Anders Lindqvist, Patrik Nordenfelt, Ulf Malmqvist, Per Hellstrand, and Ina Nordström

Subjects

Tail, medicine.medical_specialty, Time Factors, Vascular smooth muscle, Physiology, Calponin, Myosins, Organ culture, Muscle, Smooth, Vascular, Capillary Permeability, Rats, Sprague-Dawley, Contractility, Organ Culture Techniques, Internal medicine, Myosin, medicine, Animals, Cytoskeleton, Escin, Smooth muscle tissue, biology, Calcium-Binding Proteins, Microfilament Proteins, Arteries, Intracellular Membranes, Cell Biology, Calcium Channel Blockers, Fetal Blood, Rats, medicine.anatomical_structure, Endocrinology, Verapamil, Vasoconstriction, biology.protein, Biophysics, Calcium, Cattle, Female, lipids (amino acids, peptides, and proteins), medicine.symptom, Muscle contraction

Abstract

Culture of dispersed smooth muscle cells is known to cause rapid modulation from the contractile to the synthetic cellular phenotype. However, organ culture of smooth muscle tissue, with maintained extracellular matrix and cell-cell contacts, may facilitate maintenance of the contractile phenotype. To test the influence of culture conditions, structural, functional, and biochemical properties of rat tail arterial rings were investigated after culture. Rings were cultured for 4 days in the absence and presence of 10% FCS and then mounted for physiological experiments. Intracellular Ca2+concentration ([Ca2+]i) after stimulation with norepinephrine was similar in rings cultured with and without FCS, whereas force development after FCS was decreased by >50%. The difference persisted after permeabilization with β-escin. These effects were associated with the presence of vasoconstrictors in FCS and were dissociated from its growth-stimulatory action. FCS treatment increased lactate production but did not affect ATP, ADP, or AMP contents. The contents of actin and myosin were decreased by culture but similar for all culture conditions. There was no effect of FCS on calponin contents or myosin SM1/SM2 isoform composition, nor was there any appearance of nonmuscle myosin. FCS-stimulated rings showed evidence of cell degeneration not found after culture without FCS or with FCS + verapamil (1 μM) to lower [Ca2+]i. The decreased force-generating ability after culture with FCS is thus associated with increased [Ca2+]iduring culture and not primarily caused by growth-associated modulation of cells from the contractile to the synthetic phenotype.

Published

1999

5. PYK2 selectively mediates signals for growth versus differentiation in response to stretch of spontaneously active vascular smooth muscle

Author

Mario Grossi, Sebastian Albinsson, Leonard Buckbinder, Ina Nordström, Per Hellstrand, Karolina M. Turczyńska, and Anirban Bhattachariya

Subjects

medicine.medical_specialty, Vascular smooth muscle, DNA synthesis, medicine.drug_class, Physiology, contraction, chemistry.chemical_element, Calcium channel blocker, Biology, Calcium, Organ culture, Cirazoline, PF‐4594755, chemistry.chemical_compound, Endocrinology, chemistry, Physiology (medical), Internal medicine, ion channel, medicine, Phosphorylation, stretch, Protein kinase B, Original Research

Abstract

Stretch of vascular smooth muscle stimulates growth and proliferation as well as contraction and expression of contractile/cytoskeletal proteins, all of which are also regulated by calcium‐dependent signals. We studied the role of the calcium‐ and integrin‐activated proline‐rich tyrosine kinase 2 (PYK2) in stretch‐induced responses of the rat portal vein loaded by a hanging weight ex vivo. PYK2 phosphorylation at Tyr‐402 was increased both by a 10‐min stretch and by organ culture with load over several days. Protein and DNA synthesis were reduced by the novel PYK2 inhibitor PF‐4594755 (0.5–1 μmol/L), while still sensitive to stretch. In 3‐day organ culture, PF‐4594755 caused maintained myogenic spontaneous activity but did not affect contraction in response to high‐K+ (60 mmol/L) or to α1‐adrenergic stimulation by cirazoline. Basal and stretch‐induced PYK2 phosphorylation in culture were inhibited by PF‐4594755, closely mimicking inhibition of non‐voltage‐dependent calcium influx by 2‐APB (30 μmol/L). In contrast, the L‐type calcium channel blocker, nifedipine (1 μmol/L) eliminated stretch‐induced but not basal PYK2 phosphorylation. Stretch‐induced Akt and ERK1/2 phosphorylation was eliminated by PF‐4594755. PYK2 inhibition had no effect on mRNA expression of several smooth muscle markers, and stretch‐sensitive SM22α synthesis was preserved. Culture of portal vein with the Ang II inhibitor losartan (1 μmol/L) eliminated stretch sensitivity of PYK2 and Akt phosphorylation, but did not affect mRNA expression of smooth muscle markers. The results suggest that PYK2 signaling functionally distinguishes effects of voltage‐ and non‐voltage‐dependent calcium influx. A small‐molecule inhibitor of PYK2 reduces growth and DNA synthesis but does not affect contractile differentiation of vascular smooth muscle., We studied the role of the calcium‐ and integrin‐activated proline‐rich tyrosine kinase 2 (PYK2) in stretch‐induced responses of the rat portal ex vivo. PYK2 phosphorylation at Tyr‐402 was increased both by a 10‐min stretch and by organ culture under stretch for 3 days. Protein and DNA synthesis were reduced by the novel PYK2 inhibitor PF‐4594755 (0.5–1 μmol/L), but contractile differentiation was not affected. Basal and stretch‐induced PYK2 phosphorylation in culture were inhibited by PF‐4594755, closely mimicking inhibition of non‐voltage‐dependent calcium influx by 2‐APB (30 μmol/L). In contrast, the L‐type calcium channel blocker, nifedipine (1 μmol/L) eliminated stretch‐induced but not basal PYK2 phosphorylation. The results suggest that PYK2 signaling functionally distinguishes effects of voltage‐ and non‐voltage‐dependent calcium influx.

Published

2014

6. Novel blocker of NFAT activation inhibits IL-6 production in human myometrial arteries and reduces vascular smooth muscle cell proliferation

Author

Marie-Louise Lydrup, Per Hellstrand, Maria F. Gomez, Zhengwu Sun, Lisa M. Nilsson, Jenny Nilsson, Dag Wide-Swensson, Yung-Wu Chen, Ina Nordström, and Jeffery D. Molkentin

Subjects

medicine.medical_specialty, Cell type, Vascular smooth muscle, Physiology, medicine.medical_treatment, Myocytes, Smooth Muscle, Biology, contractility, Muscle, Smooth, Vascular, Cyclosporin a, Internal medicine, Obstetrics, Gynecology and Reproductive Medicine, medicine, Humans, Cells, Cultured, Dose-Response Relationship, Drug, NFATC Transcription Factors, Cell growth, Interleukin-6, Ca2+/calcineurin, NFAT, Cell Biology, Arteries, differentiation, Basic Medicine, Cell biology, Calcineurin, cyclosporin A, Endocrinology, Cytokine, endothelin-1, Myometrium, Pyrazoles, Female, Surgery, Signal transduction, Signal Transduction

Abstract

The calcineurin/nuclear factor of activated T cells (NFAT) signaling pathway has been found to play a role in regulating growth and differentiation in several cell types. However, the functional significance of NFAT in the vasculature is largely unclear. Here we show that NFATc1, NFATc3, and NFATc4 are expressed in human myometrial arteries. Confocal immunofluorescence and Western blot analysis revealed that endothelin-1 efficiently increases NFATc3 nuclear accumulation in native arteries. Endothelin-1 also stimulates NFAT-dependent transcriptional activity, as shown by a luciferase reporter assay. Both the agonist-induced NFAT nuclear accumulation and transcriptional activity were prevented by the calcineurin inhibitor CsA and by the novel NFAT blocker A-285222. Chronic inhibition of NFAT significantly reduced IL-6 production in intact myometrial arteries and inhibited cell proliferation in vascular smooth muscle cells cultured from explants from the same arteries. Furthermore, by using small interfering RNA-mediated reduction of NFATc3, we show that this isoform is involved in the regulation of cell proliferation. Protein synthesis in intact arteries was investigated using autoradiography of [35S]methionine incorporation in serum-free culture. Inhibition of NFAT signaling did not affect overall protein synthesis or specifically the synthesis rates of major proteins associated with the contractile/cytoskeletal system. An intact contractile phenotype under these conditions was also shown by unchanged force response to depolarization or agonist stimulation. Our results demonstrate NFAT expression and activation in native human vessels and point out A-285222 as a powerful pharmacological blocker of NFAT signaling in the vasculature.

Published

2007

7. Stretch-dependent modulation of contractility and growth in smooth muscle of rat portal vein

Author

Per Hellstrand, Ina Nordström, Karl Dreja, Asad Zeidan, and Ulf Malmqvist

Subjects

DNA Replication, medicine.medical_specialty, Vascular smooth muscle, Physiology, Lactams, Macrocyclic, Muscle Proteins, Neovascularization, Physiologic, Biology, Organ culture, Muscle Development, Culture Media, Serum-Free, Muscle, Smooth, Vascular, Muscle hypertrophy, Contractility, Rats, Sprague-Dawley, Tissue culture, Organ Culture Techniques, Internal medicine, Extracellular, medicine, Benzoquinones, Animals, Enzyme Inhibitors, Flavonoids, Mitogen-Activated Protein Kinase 1, Mitogen-Activated Protein Kinase Kinases, Hyperplasia, Mitogen-Activated Protein Kinase 3, Portal Vein, Quinones, Hypertrophy, Organ Size, Fetal Blood, Culture Media, Rats, Enzyme Activation, Endocrinology, medicine.anatomical_structure, Phenotype, Rifabutin, Circulatory system, Cattle, Female, Stress, Mechanical, Mitogen-Activated Protein Kinases, Cardiology and Cardiovascular Medicine, Blood vessel, Muscle Contraction, Signal Transduction

Abstract

Abstract —Increased intraluminal pressure of the rat portal vein in vivo causes hypertrophy and altered contractility in 1 to 7 days. We have used organ cultures to investigate mechanisms involved in this adaptation to mechanical load. Strips of rat portal vein were cultured for 3 days, either undistended or loaded by a weight. Length-force relations were shifted toward longer length in stretched cultured veins compared with freshly dissected veins, whereas the length-force relations of unstretched cultured veins were shifted in the opposite direction. This occurred after culture either with or without 10% FCS to promote growth. The wet weight of loaded veins increased by 56% in the presence of FCS, whereas that of undistended control veins increased by 24%. No weight increase was seen in serum-free culture. The dry/wet weight ratio decreased during culture with FCS but was not affected by stretch. Electron microscopy revealed increased cell cross-sectional area in stretched relative to unstretched veins, and protein contents were greater, as were [ 3 H]thymidine and [ 3 H]leucine incorporation rates. Growth responses were associated with the activation of stretch-sensitive extracellular signal–regulated kinases 1 and 2 and were inhibited by herbimycin A and PD 98059, inhibitors of extracellular signal–regulated kinases 1 and 2. The results demonstrate that by culture of whole vascular tissue, smooth muscle cells are maintained in the contractile phenotype and respond to stretch with a physiological adaptation involving hypertrophy/hyperplasia and remodeling of the contractile system, similar to that in vivo. Mechanical stimulation and growth factors are both required for functionally significant growth.

Published

2000

8. Differential actions of exogenous and intracellular spermine on contractile activity in smooth muscle of rat portal vein

Author

Ina Nordström, Maria F. Gomez, Bengt-Olof Nilsson, Per Hellstrand, and R Santiago Carrilho

Subjects

medicine.medical_specialty, Vascular smooth muscle, Fura-2, Physiology, Spermine, Biology, In Vitro Techniques, Muscle, Smooth, Vascular, Rats, Sprague-Dawley, chemistry.chemical_compound, Phenylephrine, Internal medicine, Extracellular, medicine, Animals, Escin, Portal Vein, Rats, Electrophysiology, Calcium Channel Agonists, Endocrinology, chemistry, Calcium, Female, medicine.symptom, Polyamine, Microelectrodes, Intracellular, Muscle contraction, medicine.drug, Muscle Contraction

Abstract

Effects of the naturally occurring polyamine spermine on electrical and contractile properties of the rat portal vein were studied. 1 mM spermine nearly abolished spike activity and spontaneous contractions and decreased the intracellular Ca2+ concentration ([Ca2+]i). The phasic force responses to 0.1 and 1 microM phenylephrine were partially inhibited, but not the sustain plateau contraction caused by 5 microM phenylephrine. The Ca(2+)-force relation in high-K+ (128 mM)-depolarized veins was shifted to the right, EC50 for Ca2+ increasing from 0.50 +/- 0.03 mM (control, n = 8) to 0.65 +/- 0.06 and to 0.94 +/- 0.03 at 1 (n = 4) and 10 (n = 3) mM spermine, respectively. However, at a Ca2+ concentration of 2.5 mM, giving maximal force, there was no effect of spermine (1 mM) on either force or [Ca2+]i. Whereas extracellular spermine thus reduced contractile activity at moderate levels of stimulation, increased intracellular concentration of spermine potentiated the force response to Ca2+. Intracellular loading of spermine by reversible permeabilization increased its concentration by 2-3 times. The spontaneous activity and response to phenylephrine were unchanged. However, the Ca(2+)-force relation of depolarized veins was shifted to the left, EC50 decreasing from 0.51 +/- 0.04 mM in controls (n = 7) to 0.36 +/- 0.02 mM in the loaded veins (n = 9). Spermine increased Ca(2+)-activated force in portal veins permeabilized with beta-escin. The degree of potentiation was consistent with observed effects in spermine-loaded intact veins. The results suggest that spermine at physiological intracellular concentration may contribute to the determination of Ca2+ sensitivity in vascular smooth muscle cells.

Published

1995

9. Ablation of SM22α decreases contractility and actin contents of mouse vascular smooth muscle

Author

Per Hellstrand, Karl Swärd, Eva Ekblad, Asad Zeidan, Michael S. Parmacek, Ina Nordström, and Janet C.L. Zhang

Subjects

medicine.medical_specialty, Vascular smooth muscle, Calponin, Biophysics, Muscle Proteins, Alpha (ethology), Adrenergic, Mice, Inbred Strains, macromolecular substances, Biochemistry, Muscle, Smooth, Vascular, Contractility, Mice, Structural Biology, Receptors, Adrenergic, alpha-1, Internal medicine, Genetics, Protein biosynthesis, medicine, Animals, Protein Isoforms, Receptor, Molecular Biology, Actin, Mice, Knockout, biology, Stretch, Microfilament Proteins, Cell Biology, Actins, Cell biology, Resistance artery, Endocrinology, Differentiation, Portal vein, biology.protein, Blood Vessels, Adrenergic alpha-Agonists, Muscle Contraction

Abstract

The actin-binding protein SM22alpha marks contractile differentiation in smooth muscle, but its function is unknown. We tested its role in arterial contractility and stretch-sensitive vascular protein synthesis. Active stress in depolarised mesenteric resistance arteries and portal veins was reduced by 40% in SM22alpha(-/-) mice. Passive and active arterial circumference-force relationships were shifted leftwards, whereas alpha(1)-adrenergic responses were increased. Actin contents were 10-25% lower in vessels from SM22alpha(-/-) mice, but protein composition was otherwise similar. Synthesis of SM22alpha, calponin and alpha-actin, but not beta-actin, was sensitive to stretch. Ablation of SM22alpha did not affect stretch sensitivity of any of these proteins. Thus, SM22alpha plays a role in contractility, possibly by affecting actin filament organisation.