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1. Effects of renal sympathetic denervation and angiotensin-converting enzyme inhibitor on left ventricular hypertrophy.

Author

Ding, X., Xu, X., Yan, Y., Song, X., Liu, S., Wang, G., Su, D., Jing, Q., and Qin, Y.

Abstract

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Published
2015
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2. Human Parainfluenza Virus Infection of the Airway Epithelium: Viral Hemagglutinin-Neuraminidase Regulates Fusion Protein Activation and Modulates Infectivity

Author

Anne Moscona, Laura M. Palermo, Christine C. Yokoyama, Samantha G. Palmer, Stefan Niewiesk, Bruce A. Mungall, Olga Greengard, Matteo Porotto, Palermo, Laura M., Porotto, Matteo, Yokoyama, Christine C., Palmer, Samantha G., Mungall, Bruce A., Greengard, Olga, Niewiesk, Stefan, and Moscona, Anne

Subjects
Gene Expression Regulation, Viral, Paramyxoviridae, Rats, Inbred Strain, Immunology, Hemagglutinin (influenza), Biology, Microbiology, Virus, Cell Line, Virology, Receptors, Viru, Animals, Humans, HN Protein, Mononegavirales, Viral Fusion Protein, Lung, Paramyxoviridae Infections, Animal, Rats, Inbred Strains, biology.organism_classification, Paramyxoviridae Infection, Fusion protein, Parainfluenza Virus 3, Human, Rats, Cell culture, Insect Science, biology.protein, Rat, Receptors, Virus, Pathogenesis and Immunity, Female, Viral Fusion Proteins, Neuraminidase, Human
Abstract

Three discrete activities of the paramyxovirus hemagglutinin-neuraminidase (HN) protein, receptor binding, receptor cleaving (neuraminidase), and triggering of the fusion protein, each affect the promotion of viral fusion and entry. For human parainfluenza virus type 3 (HPIV3), the effects of specific mutations that alter these functions of the receptor-binding protein have been well characterized using cultured monolayer cells, which have identified steps that are potentially relevant to pathogenesis. In the present study, proposed mechanisms that are relevant to pathogenesis were tested in natural host cell cultures, a model of the human airway epithelium (HAE) in which primary HAE cells are cultured at an air-liquid interface and retain functional properties. Infection of HAE cells with wild-type HPIV3 and variant viruses closely reflects that seen in an animal model, the cotton rat, suggesting that HAE cells provide an ideal system for assessing the interplay of host cell and viral factors in pathogenesis and for screening for inhibitory molecules that would be effective in vivo. Both HN's receptor avidity and the function and timing of F activation by HN require a critical balance for the establishment of ongoing infection in the HAE, and these HN functions independently modulate the production of active virions. Alterations in HN's F-triggering function lead to the release of noninfectious viral particles and a failure of the virus to spread. The finding that the dysregulation of F triggering prohibits successful infection in HAE cells suggests that antiviral strategies targeted to HN's F-triggering activity may have promise in vivo. Copyright © 2009, American Society for Microbiology. All Rights Reserved.

Published
2009
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3. Relationships among alterations in renal membrane sodium transport, renin and aminopeptidase M activities in genetic hypertension

Author

Paolo Parenti, Chiara Troffa, B. R. Barber, Sergio Salardi, Rocco Falchetto, Sabrina Pastore, Giuseppe Bianchi, Nicola Glorioso, Salardi, S, Falchetto, R, Troffa, C, Parenti, P, Barber, B, Pastore, S, Glorioso, N, and Bianchi, G

Subjects
medicine.medical_specialty, Hypertension, Renal, Kidney Cortex, Rats, Inbred Strain, Aminopeptidase, Sodium, Antigens, CD13, chemistry.chemical_element, Blood Pressure, CD13 Antigens, Aminopeptidases, Plasma renin activity, law.invention, chemistry.chemical_compound, law, Internal medicine, Renin, Renin–angiotensin system, medicine, Animals, Electrophoresis, Gel, Two-Dimensional, Molecular Biology, Kinetic, chemistry.chemical_classification, Kidney, Microvilli, Animal, Rats, Inbred Strains, Biological Transport, BIO/10 - BIOCHIMICA, Rats, Kinetics, Endocrinology, medicine.anatomical_structure, Enzyme, chemistry, Recombinant DNA, Rat, Molecular Medicine, PMSF
Abstract

Rats of the Milan Hypertensive Strain (MHS) may be considered a useful model for understanding the genetic molecular mechanism underlying a primary form of hypertension in at least a subgroup of patients. Many differences between MHS and its normotensive control strain (MNS) were found at the organ, cellular and biochemical level. In the present investigation renal cell membrane proteins (BBMV) were analysed by two-dimensional electrophoresis and a difference between MHS and MNS was shown in a polypeptide of 32 kDa, subsequently identified as the C-terminal fragment of aminopeptidase M (APM). The activity of the enzyme was higher in MHS. Genetic relationships between this enzyme and the other biochemical cellular abnormalities of MHS, namely sodium transport in BBMV and renin activity in kidney cortex were investigated in MHS, MNS and in two inbred recombinant strains. This analysis showed that faster sodium transport, low kidney levels of renin and hypertension, but not differences in two-dimensional electrophoretic pattern and in aminopeptidase M activity, cosegregated in recombinant strains. These results are consistent with the hypothesis that the faster sodium transport can be considered a primary cellular abnormality responsible for hypertension in MHS and that the aminopeptidase difference is not involved in the cellular abnormalities.

Published
1993
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4. Na+,2Cl−,K+ cotransport system as a marker of antihypertensive activity of new torasemide derivatives

Author

Bernard Masereel, Jacques Delarge, Marra Ferrandi, Bernard Pirotte, Marc Schynts, Paolo Parenti, Patrizia Ferrari, Masereel, B, Ferrari, P, Ferrandi, M, Pirotte, B, Schynts, M, Parenti, P, and Delarge, J

Subjects
Male, medicine.medical_specialty, Erythrocytes, Rats, Inbred Strain, medicine.drug_class, medicine.medical_treatment, Blood Pressure, In Vitro Techniques, Sulfonamide, Structure-Activity Relationship, Rats, Inbred SHR, Internal medicine, medicine, Animals, Diuretic, Potency, Diuretics, IC50, Bumetanide, Pharmacology, Sulfonamides, Kidney Medulla, Kidney, Animal, Chemistry, Sodium, Rats, Inbred Strains, Rubidium Radioisotope, Loop diuretic, Torsemide, BIO/10 - BIOCHIMICA, Rats, Erythrocyte, Red blood cell, Endocrinology, medicine.anatomical_structure, Hypertension, Potassium, Rat, Chlorine, Cotransporter, Rubidium Radioisotopes, medicine.drug
Abstract

A series of compounds related to torasemide, a loop diuretic, were synthesized and examined for their diuretic potency and inhibitory activity on the erythrocyte and renal medullary thick ascending limb vesicle Na+,2Cl-,K+ cotransport in Milan hypertensive (MHS) and normotensive (MNS) rat strains, where previous studies had demonstrated an alteration of the cotransport system genetically related to hypertension. From the results of the screening, structure-activity relationships were drawn and two compounds, JDL 961 and C 2921 were selected. Their IC50 on renal vesicle cotransport were similar in the two strains (JDL 961: MHS = 1.8 microM; MNS = 1.2 microM; C 2921: MHS = 4 microM; MNS = 3.8 microM), and were 4-8 times lower than those of torasemide (MHS = 13 microM; MNS = 31 microM, P less than 0.01) and 50-60 times lower than those of bumetanide (MHS = 145 microM; MNS = 206 microM, P less than 0.05) taken as reference compounds. Their ability to reduce the development rate of hypertension was tested both in MHS and in Okamoto spontaneously hypertensive rats (SHR) strain, in which cotransport alterations are opposite to those of MHS. Both torasemide derivatives (7.5 mg.kg-1 os per day) prevented development of hypertension in the two strains. The time course of this hypotensive activity was faster and the percentage of blood pressure fall greater in MHS (20-25%) than in SHR rats (12-15%), even though the absolute value of blood pressure fall was similar in MHS (JDL 961 = -17 mm Hg; C 2921 = -30 mm Hg) and SHR (JDL 961 = -25 mm Hg; C 2921 = -20 mm Hg). A superimposable effect of bumetanide was observed in the two strains, but at 8 times higher daily dose (60 mg.kg-1). These results suggest that new loop diuretics can be selected for their antihypertensive activity on the basis of their in vitro potency in inhibiting the Na+,2Cl-,K+.

Published
1992
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5. Diabetes-induced alteration of HMGCoA reductase forms in rat livers

Author

Fulvio Magni, M. Galli Kienle, M. Cancellieri, M. Del Puppo, Magni, F, Cancellieri, M, DEL PUPPO, M, and Galli Kienle, M

Subjects
Blood Glucose, Male, medicine.medical_specialty, Rats, Inbred Strain, Endocrinology, Diabetes and Metabolism, Coenzyme A, Biology, Reductase, Hydroxymethylglutaryl CoA Reductase, Diabetes Mellitus, Experimental, chemistry.chemical_compound, Endocrinology, Reference Values, Diabetes mellitus, Internal medicine, Internal Medicine, medicine, Animals, Reference Value, Phosphorylation, chemistry.chemical_classification, Animal, Rats, Inbred Strains, General Medicine, Glutathione, medicine.disease, Streptozotocin, Hydroxymethylglutaryl-CoA reductase, Isoenzyme, Rats, Isoenzymes, Enzyme, Liver, chemistry, Microsomes, Liver, Rat, Hydroxymethylglutaryl CoA Reductases, Specific activity, medicine.drug
Abstract

The effects of streptozotocin-induced diabetes on the various forms of 3-hydroxy-3-methylglutaryl coenzyme A reductase (HMGCoA reductase), phosphorylated/dephosphorylated and thiolic/disulphide, were studied in rat liver. Animals were treated twice with 65 mg/kg intraperitoneally of streptozotocin to induce diabetes and sacrificed after 5 days. The relative amounts of the four possible forms of the enzyme were determined in control and diabetic rats. As determined from the total activity, and in agreement with previous reports, the enzyme protein was significantly decreased in streptozotocin-treated rats. However, the percentage of the active thiolic dephosphorylated form was higher in these animals than in controls, suggesting a response of the liver to the decrease both total and specific activity of HMGCoA reductase.

Published
1992
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6. Calcium signaling and secretory responses in agonist-stimulated pituitary gonadotrophs

Author

Eduardo Rojas, Toshihiko Iida, Kevin J. Catt, Antonio Torsello, Stanko S. Stojilkovic, Stojilković, S, Torsello, A, Iida, T, Rojas, E, and Catt, K

Subjects
Rats, Inbred Strain, Endocrinology, Diabetes and Metabolism, Clinical Biochemistry, Gonadotropin-releasing hormone, Biochemistry, Calcium in biology, Membrane Potentials, Gonadotropin-Releasing Hormone, Endocrinology, Reference Values, Reference Value, Cells, Cultured, Protein Kinase C, Voltage-dependent calcium channel, Cobalt, Calcium Channel Blockers, Perfusion, Tetradecanoylphorbol Acetate, Molecular Medicine, Female, Calcium Channel Blocker, hormones, hormone substitutes, and hormone antagonists, Signal Transduction, endocrine system, medicine.medical_specialty, Ovariectomy, chemistry.chemical_element, Biology, Calcium, Gonadotropic cell, Calcium Channel, Membrane Potential, Exocytosis, Pituitary Gland, Anterior, Internal medicine, Extracellular, medicine, Animals, Molecular Biology, Protein kinase C, Kinetic, Animal, Rats, Inbred Strains, Cell Biology, 3-Pyridinecarboxylic acid, 1,4-dihydro-2,6-dimethyl-5-nitro-4-(2-(trifluoromethyl)phenyl)-, Methyl ester, Luteinizing Hormone, Rats, Kinetics, chemistry, Potassium, Rat, Calcium Channels
Abstract

In cultured pituitary gonadotrophs, gonadotropin-releasing hormone (GnRH) caused dose-dependent and biphasic increases in cytoplasmic calcium concentration ([Ca2+]i) and LH release. Both extra- and intracellular calcium pools participate in GnRH-induced elevation of [Ca2+]i and LH secretion. The spike phase of the [Ca2+]i response represents the primary signal derived predominantly from the rapid mobilization of intracellular Ca2+. In contrast, the prolonged phase of the Ca2+ signal depends exclusively on Ca2+ entry from the extracellular pool. The influx of Ca2+ occurs partially through dihydropyridine-sensitive calcium channels. Both [Ca2+]i and LH responses to increasing concentrations of GnRH occur over very similar time scales, suggesting that increasing degrees of receptor occupancy are transduced into amplitude-modulated Ca2+ responses, which in turn activate exocytosis in a linear manner. However, several lines of evidence indicated the complexity over the relationship between Ca2+ signaling and LH exocytosis. In contrast to [Ca2+]i measurements in cell suspension, single cell Ca2+ measurements revealed the existence of a more complicated pattern of Ca2+ response to GnRH, with a biphasic response to high agonist doses and prominent oscillatory responses to lower GnRH concentrations, with a log-linear correlation between GnRH dose and the frequency of Ca2+ spiking. In addition, analysis of the magnitudes of the [Ca2+]i and LH responses of gonadotrophs to a wide range of GnRH concentrations in the presence and absence of extracellular Ca2+, and to K+ and phorbol ester stimulation, showed non-linearity between these parameters with amplification of [Ca2+]i-mediated exocytosis. Studies on cell depleted of protein kinase C under conditions that did not change the LH pool suggested the participation of protein kinase C in this amplification, especially during the plateau phase of the secretory response to GnRH.

Published
1992
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7. Na+/K+/Cl−-cotransporter mediated Rb+ fluxes in membrane vesicles from kidneys of normotensive and hypertensive rats

Author

Giuseppe Bianchi, Sergio Salardi, Paolo Parenti, Mara Ferrandi, R. Braw, Paolo Ferrari, Steven J.D. Karlish, Ferrandi, M, Salardi, S, Parenti, P, Ferrari, P, Bianchi, G, Braw, R, and Karlish, S

Subjects
Male, medicine.medical_specialty, Rats, Inbred Strain, Biophysics, Diaphragm pump, In Vitro Techniques, Kidney, Chloride, Rats, Inbred WKY, Biochemistry, Chlorides, Furosemide, Microsomes, Rats, Inbred SHR, Internal medicine, medicine, Renal medulla, Na-K-Cl cotransporter, Animals, Na+/K+-ATPase, Ion transporter, biology, Animal, Chemistry, Sodium, Microsome, Rats, Inbred Strains, Biological Transport, Cell Biology, Rubidium, BIO/10 - BIOCHIMICA, Rats, Endocrinology, medicine.anatomical_structure, Hypertension, Potassium, biology.protein, Rat, Cotransporter, Bumetanide, medicine.drug
Abstract

This paper describes experiments to examine Rb + fluxes via the Na + /K + /Cl − cotransporter in membrane vesicles from renal outer medulla of three strains of rat: (A) Wistar (B) Milan hypertensive (MHS) and normotensive (MNS), and (C) Sabra salt-sensitive hypertensive (SBH) and salt-resistant (SBN). Initially, Na + -dependent furosemide- or bumetanide-inhibited 86 Rb + fluxes were characterised using Wistar rat microsomes. The latter were partially purified on a metrizamide cushion, and assay conditions were optimized for use with microsomes from the other rats. The major result is that in microsomes from adult Milan hypetensive (MHS) rats the rate of the Na + /K + /Cl − -cotransporter mediated 86 Rb flux at sub-saturating concentrations of Rb, appears to be significantly greater than in the normotensive (MNS) controls. The effect reflects an increased apparent Rb affinity of the cotransporter in MHS microsomes. There is no difference in maximal rate or in the apparent Na + activation affinity of the 86 Rb + flux. In addition bumetanide appears to be a somewhat more effective inhibitor in MHS compared to MNS microsomes. The 86 Rb + flux result is compatible with a previous finding that in red cells, Na + /K + -cotransporter mediated fluxes are increased in MHS compared to MNS. It supports the notion that the Na + /K + /Cl − -cotransporter in both red cells and kidney is a genetic marker for hypertension. It is of interest that apparetly more than one Na + transport system is affected in MHS hypertensive kidneys (a) the Na + /K + /Cl − cotransporter i nthe thick ascending limb of Henle and (b) the Na + /H + exchanger and/or a conductive Na + -pathway in brush-border membranes from proximal tubule. It is conceivable that in the hypertensive animals a common regulatory pathway (e.g., phosphorylation) or protein (e.g., cytoskeleton) is affected along the length of the nephron. In Sabra SBH and SBN rat microsomes, no difference was found for the 86 Rb + flux via the Na + /K + /Cl − cotransporter (or via a K + channel).

Published
1990
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8. Asymmetric synthesis and preliminary evaluation of (R)- and (S)-[11C]bisoprolol, a putative beta1-selective adrenoceptor radioligand

Author

P. Simonelli, Thomas A. Bonasera, Marzia Galli Kienle, A. Carpinelli, Francesco Sudati, Diego Colombo, Mario Matarrese, Rosa Maria Moresco, Sergio Todde, Fulvio Magni, Ferruccio Fazio, Dmitri Soloviev, Soloviev, D, Matarrese, M, Moresco, R, Todde, S, Bonasera, T, Sudati, F, Simonelli, P, Magni, F, Colombo, D, Carpinelli, A, Kienle, M, and Fazio, F

Subjects
Male, Stereochemistry, Rats, Inbred Strain, Ligand, Propranolol, Ligands, Cellular and Molecular Neuroscience, chemistry.chemical_compound, In vivo, Receptors, Adrenergic, beta, Radioligand, medicine, Animals, Bisoprolol, Tissue Distribution, Lung, MED/36 - DIAGNOSTICA PER IMMAGINI E RADIOTERAPIA, Sodium cyanoborohydride, Animal, Myocardium, Radiosynthesis, Brain, Rats, Inbred Strains, Stereoisomerism, Cell Biology, BIO/10 - BIOCHIMICA, Rats, chemistry, Rat, Stereoselectivity, Enantiomer, medicine.drug
Abstract

(+/-)-1-[4-(2-Isopropoxyethoxymethyl)-phenoxy]-3-isopropylamino-2-propanol (bisoprolol) is a potent, clinically used beta(1)-adrenergic agent. (R)-(+) and (S)-(-) enantiomers of bisoprolol were labelled with carbon-11 (t(1/2)=20.4 min) as putative tracers for the non-invasive assessment of the beta(1)-adrenoceptor subtype in the human heart and brain with positron emission tomography (PET). The radiosynthesis consisted of reductive alkylation of des-iso-propyl precursor with [2-11C]acetone in the presence of sodium cyanoborohydride and acetic acid. The stereo-conservative synthesis of (R)-(+) and (S)-(-)-1-[4-(2-isopropoxyethoxymethyl)-phenoxy]-3-amino-2-propanol to be used as the precursors for the radiosynthesis of [11C]bisoprolol enantiomers was readily accomplished by the use of the corresponding chiral epoxide in three steps starting from the commercially available hydroxybenzyl alcohol. The final labelled product (either (+) or (-)-1-[4-(-isopropoxyethoxymethyl)-phenoxy]-3- [11C]isopropylamino-2-propanol) was obtained in 99% radiochemical purity in 30 min with 15+/-5% (EOS, non-decay corrected) radiochemical yield and 3.5+/-1 Ci/micromol specific radioactivity. Preliminary biological evaluation of the tracer in rats showed that about 30% of heart uptake of [11C](S)-bisoprolol is due to specific binding. The high non-specific uptake in lung might mask the heart uptake, thus precluding the use of [11C](S)-bisoprolol for heart and lung studies by PET. The remarkably high uptake of the tracer in rat brain areas rich of beta-adrenergic receptors such as pituitary (1.8+/-0.3% I.D. at 30 min) was blocked by pre-treatment with the beta-adrenergic antagonists propranolol (45%) and bisoprolol (51%, p

Published
2001

9. Asymmetric synthesis and preliminary evaluation of (R)- and (S)-[11C]bisoprolol, a putative beta1-selective adrenoceptor radioligand

Author

Soloviev, D, Matarrese, M, Moresco, R, Todde, S, Bonasera, T, Sudati, F, Simonelli, P, Magni, F, Colombo, D, Carpinelli, A, Kienle, M, Fazio, F, Soloviev, DV, MORESCO, ROSA MARIA, TODDE, SERGIO CAMILLO, Bonasera, TA, MAGNI, FULVIO, KIENLE, MARZIA DONATELLA, FAZIO, FERRUCCIO, Soloviev, D, Matarrese, M, Moresco, R, Todde, S, Bonasera, T, Sudati, F, Simonelli, P, Magni, F, Colombo, D, Carpinelli, A, Kienle, M, Fazio, F, Soloviev, DV, MORESCO, ROSA MARIA, TODDE, SERGIO CAMILLO, Bonasera, TA, MAGNI, FULVIO, KIENLE, MARZIA DONATELLA, and FAZIO, FERRUCCIO

Abstract

(+/-)-1-[4-(2-Isopropoxyethoxymethyl)-phenoxy]-3-isopropylamino-2-propanol (bisoprolol) is a potent, clinically used beta(1)-adrenergic agent. (R)-(+) and (S)-(-) enantiomers of bisoprolol were labelled with carbon-11 (t(1/2)=20.4 min) as putative tracers for the non-invasive assessment of the beta(1)-adrenoceptor subtype in the human heart and brain with positron emission tomography (PET). The radiosynthesis consisted of reductive alkylation of des-iso-propyl precursor with [2-11C]acetone in the presence of sodium cyanoborohydride and acetic acid. The stereo-conservative synthesis of (R)-(+) and (S)-(-)-1-[4-(2-isopropoxyethoxymethyl)-phenoxy]-3-amino-2-propanol to be used as the precursors for the radiosynthesis of [11C]bisoprolol enantiomers was readily accomplished by the use of the corresponding chiral epoxide in three steps starting from the commercially available hydroxybenzyl alcohol. The final labelled product (either (+) or (-)-1-[4-(-isopropoxyethoxymethyl)-phenoxy]-3- [11C]isopropylamino-2-propanol) was obtained in 99% radiochemical purity in 30 min with 15+/-5% (EOS, non-decay corrected) radiochemical yield and 3.5+/-1 Ci/micromol specific radioactivity. Preliminary biological evaluation of the tracer in rats showed that about 30% of heart uptake of [11C](S)-bisoprolol is due to specific binding. The high non-specific uptake in lung might mask the heart uptake, thus precluding the use of [11C](S)-bisoprolol for heart and lung studies by PET. The remarkably high uptake of the tracer in rat brain areas rich of beta-adrenergic receptors such as pituitary (1.8+/-0.3% I.D. at 30 min) was blocked by pre-treatment with the beta-adrenergic antagonists propranolol (45%) and bisoprolol (51%, p<0.05). [11C](S)-bisoprolol deserves further evaluation in other animal models as a putative beta(1) selective radioligand for in vivo investigation of central adrenoceptors.

Published
2001

10. Effect of different regimens of gut decontamination on bacterial translocation and mortality in experimental acute pancreatitis

Author

Gianotti, L, Munda, R, Gennari, R, Pyles, R, Alexander, J, GIANOTTI, LUCA VITTORIO, Alexander, J., Gianotti, L, Munda, R, Gennari, R, Pyles, R, Alexander, J, GIANOTTI, LUCA VITTORIO, and Alexander, J.

Abstract

To assess the effect of four regimens of antibiotics (compared with a control regimen of distilled water) given orally on gut decontamination, bacterial translocation, and mortality in acute necrotising pancreatitis in mice

Published
1995

11. Steroids and tissue-specific modulation of galanin gene expression in the male rat reproductive system

Author

Jean-Claude Vuille, C Ikejiani, I. C. Schroedter, Maria Vrontakis, Henry G. Friesen, A Torsello, Torsello, A, Vrontakis, M, Schroedter, I, Vuille, J, Ikejiani, C, and Friesen, H

Subjects
Male, endocrine system, medicine.medical_specialty, Transcription, Genetic, medicine.drug_class, Rats, Inbred Strain, Colon, medicine.medical_treatment, Adrenal Gland, Neuropeptide, Hypothalamus, Middle, Gene Expression, Galanin, In situ hybridization, Thymus Gland, Biology, Genitalia, Male, Dexamethasone, Endocrinology, Internal medicine, Adrenal Glands, medicine, Animals, RNA, Messenger, Diethylstilbestrol, Animal, Neuropeptides, digestive, oral, and skin physiology, Vas deferens, Rats, Inbred Strains, Dihydrotestosterone, Androgen, Epididymis, Rats, Steroid hormone, medicine.anatomical_structure, nervous system, Gene Expression Regulation, Hypothalamus, Organ Specificity, Peptide, Rat, Peptides, hormones, hormone substitutes, and hormone antagonists
Abstract

Galanin is a neuropeptide widely distributed throughout the vertebrate neural and endocrine system. Galanin can influence pituitary hormone secretion, intestinal motility, and other biological activities. The precise physiological role of galanin is unknown. We studied the control of galanin gene expression in peripheral organs in the male rat using Northern blot and in situ hybridization techniques. In the adrenals and prostate, galanin mRNA was undetectable in the controls and did not change after the administration of dexamethasone (0.0001-10.0 mg/kg, ip) and diethylstilbestrol (0.1 mg/kg, ip). In the testis, thymus, seminal vesicles, medial basal hypothalamus, and colon, galanin message was detectable, but was not influenced by steroids. On the other hand, dexamethasone (0.5-10.0 mg/kg) was very effective in enhancing galanin expression in the vas deferens and epididymis (4- to 7-fold in the vas deferens), with a peak 6-9 h after the treatment. Diethylstilbestrol (0.1 mg/kg) stimulated galanin mRNA transcription only in the vas deferens (2- to 3-fold), with a peak 1-3 h after the treatment. Dihydrotestosterone treatment (0.2-0.4 mg/kg) was ineffective in all tissues examined. In the vas deferens and seminal vesicles, galanin mRNA has been localized at a cellular level by in situ hybridization. In these tissues only fibroblast-like cells contained the message. These data demonstrate that galanin is expressed in the male rat reproductive system and that steroid hormones participate in the control of galanin gene expression in a tissue- and hormone-specific fashion.

Published
1992

12. Relationships among alterations in renal membrane sodium transport, renin and aminopeptidase M activities in genetic hypertension

Author

Salardi, S, Falchetto, R, Troffa, C, Parenti, P, Barber, B, Pastore, S, Glorioso, N, Bianchi, G, PARENTI, PAOLO, Barber, BR, Bianchi, G., Salardi, S, Falchetto, R, Troffa, C, Parenti, P, Barber, B, Pastore, S, Glorioso, N, Bianchi, G, PARENTI, PAOLO, Barber, BR, and Bianchi, G.

Abstract

Rats of the Milan Hypertensive Strain (MHS) may be considered a useful model for understanding the genetic molecular mechanism underlying a primary form of hypertension in at least a subgroup of patients. Many differences between MHS and its normotensive control strain (MNS) were found at the organ, cellular and biochemical level. In the present investigation renal cell membrane proteins (BBMV) were analysed by two-dimensional electrophoresis and a difference between MHS and MNS was shown in a polypeptide of 32 kDa, subsequently identified as the C-terminal fragment of aminopeptidase M (APM). The activity of the enzyme was higher in MHS. Genetic relationships between this enzyme and the other biochemical cellular abnormalities of MHS, namely sodium transport in BBMV and renin activity in kidney cortex were investigated in MHS, MNS and in two inbred recombinant strains. This analysis showed that faster sodium transport, low kidney levels of renin and hypertension, but not differences in two-dimensional electrophoretic pattern and in aminopeptidase M activity, cosegregated in recombinant strains. These results are consistent with the hypothesis that the faster sodium transport can be considered a primary cellular abnormality responsible for hypertension in MHS and that the aminopeptidase difference is not involved in the cellular abnormalities

Published
1993

13. Interactions between calcium and protein kinase C in the control of signaling and secretion in pituitary gonadotrophs

Author

Toshihiko Iida, Kevin J. Catt, Francesco Merelli, Stanko S. Stojilkovic, A Torsello, Lazar Z. Krsmanovic, Stojilković, S, Iida, T, Merelli, F, Torsello, A, Krsmanović, L, and Catt, K

Subjects
endocrine system, medicine.medical_specialty, Rats, Inbred Strain, Blotting, Western, chemistry.chemical_element, Stimulation, Gonadotropin-releasing hormone, Calcium, Biology, Gonadotropic cell, Biochemistry, Calcium Channel, Membrane Potential, Exocytosis, Membrane Potentials, Gonadotropin-Releasing Hormone, Alkaloids, Pituitary Gland, Anterior, Internal medicine, Alkaloid, medicine, Animals, Molecular Biology, BIO/14 - FARMACOLOGIA, Ion transporter, Protein kinase C, Cells, Cultured, Protein Kinase C, Voltage-dependent calcium channel, Animal, Temperature, Biological Transport, Rats, Inbred Strains, Cell Biology, Luteinizing Hormone, Staurosporine, Rats, Enzyme Activation, Endocrinology, chemistry, Biophysics, Potassium, Rat, Tetradecanoylphorbol Acetate, Female, Calcium Channels, Signal Transduction
Abstract

Single pituitary gonadotrophs exhibit episodes of spontaneous fluctuations in cytoplasmic calcium concentration [( Ca2+]i) due to entry through voltage-sensitive calcium channels (VSCC) and show prominent agonist-induced oscillations in [Ca2+]i that are generated by periodic release of intracellular Ca2+. Gonadotropin releasing hormone (GnRH) elicited three types of Ca2+ responses: at low doses, subthreshold, with an increase in basal [Ca2+]i; at intermediate doses, oscillatory, with dose-dependent modulation of spiking frequency; and at high doses, biphasic, without oscillations. Elevation of [Ca2+]i or activation of protein kinase C (PKC) did not influence the frequency of agonist-induced [Ca2+]i spikes but caused dose-dependent reductions in amplitude for all types of Ca2+ response. Stimulation of transient Ca2+ spikes by GnRH was followed by inhibition of the spontaneous fluctuations. GnRH also reduced the ability of high extracellular K+ to promote Ca2+ influx through VSCC. Activation of PKC by phorbol esters stimulated Ca2+ influx in quiescent cells but inhibited influx when VSCC were already activated, either spontaneously or by high K+. In contrast to their biphasic actions on [Ca2+]i, phorbol esters exerted only stimulatory actions on gonadotropin release, even when Ca2+ influx was concomitantly reduced. However, pituitary cells had to be primed with an appropriate [Ca2+]i level before exocytosis could be amplified by PKC. In PKC-depleted cells, all actions of phorbol esters on Ca2+ entry and amplitude modulation, and on LH release, were abolished. GnRH-induced LH secretion was also significantly reduced, especially the plateau phase of the response. These data indicate that Ca2+ and PKC serve as interacting signals during the cascade of cellular events triggered by agonist stimulation, in which Ca2+ turns cell responses on or off, and PKC amplifies the positive and negative effects of Ca2+.

Published
1991

14. Role of phosphatidylethanol in membranes. Effects on membrane fluidity, tolerance to ethanol, and activity of membrane-bound enzymes

Author

Omodeo Salé, F, Lindi, C, PALESTINI, PAOLA NOVERINA ADA, MASSERINI, MASSIMO ERNESTO, Omodeo Salé, F, Lindi, C, Palestini, P, and Masserini, M

Subjects
Male, Intracellular Membrane, Kinetic, Calorimetry, Differential Scanning, Ethanol, Animal, Membrane Fluidity, Rats, Inbred Strain, Submitochondrial Particle, Phosphatidylethanolamine, Brain, Liposome, Spectrometry, Fluorescence, Membrane Lipid, Rat, Sodium-Potassium-Exchanging ATPase, Dimyristoylphosphatidylcholine, 5'-Nucleotidase
Abstract

We investigated the effect of phosphatidylethanol (PEt) on fluidity and membrane tolerance to the fluidization induced by ethanol as well as on the activity of two membrane-bound enzymes, Na+/K+ ATPase and 5'-nucleotidase. PEt was synthesized from 1,2-dimyristoylphosphatidylcholine and phosphatidylcholine from bovine brain and studies were performed to determine the optimal experimental conditions for the insertion of PEt in natural bilayers. The effects of PEt, evaluated by differential scanning calorimetry or fluorescence polarization techniques, were studied in model membranes made of synthetic phospholipids or made of total lipids extracted from rat brain crude mitochondrial fraction (P2 fraction) and from natural membranes (P2 fraction). The presence of PEt increased the fluidity of artificial as well of natural membranes, but tolerance to the addition of ethanol, displayed by dimyristoylphosphatidylcholine vesicles and by natural membranes containing PEt, was lacking in vesicles made of dimyristoylphosphatidylethanolamine and in artificial bilayers reconstituted from total P2 lipid extracts, suggesting an involvement of PC on PEt-induced ethanol resistance. Na+/K+ ATPase activity was enhanced by the addition of small amounts of ethanol (up to 50 mM) and progressively inhibited at higher concentrations, while 5'-nucleotidase was not affected up to 400 mM ethanol. The presence of PEt in the bilayer exerted the opposite effects on the two enzymes, reducing the Na+/K+ ATPase activation induced by ethanol and enhancing 5'-nucleotidase activity. The mechanisms of the PEt-induced modifications are discussed.

Published
1991

15. Diabetes-induced alteration of HMGCoA reductase forms in rat livers

Author

Magni, F, Cancellieri, M, DEL PUPPO, M, Galli Kienle, M, MAGNI, FULVIO, DEL PUPPO, MARINA, Galli Kienle, M., Magni, F, Cancellieri, M, DEL PUPPO, M, Galli Kienle, M, MAGNI, FULVIO, DEL PUPPO, MARINA, and Galli Kienle, M.

Abstract

The effects of streptozotocin-induced diabetes on the various forms of 3-hydroxy-3-methylglutaryl coenzyme A reductase (HMGCoA reductase), phosphorylated/dephosphorylated and thiolic/disulphide, were studied in rat liver. Animals were treated twice with 65 mg/kg intraperitoneally of streptozotocin to induce diabetes and sacrificed after 5 days. The relative amounts of the four possible forms of the enzyme were determined in control and diabetic rats. As determined from the total activity, and in agreement with previous reports, the enzyme protein was significantly decreased in streptozotocin-treated rats. However, the percentage of the active thiolic dephosphorylated form was higher in these animals than in controls, suggesting a response of the liver to the decrease both total and specific activity of HMGCoA reductase.

Published
1992

16. Calcium signaling and secretory responses in agonist-stimulated pituitary gonadotrophs

Author

Stojilković, S, Torsello, A, Iida, T, Rojas, E, Catt, K, TORSELLO, ANTONIO BIAGIO, Catt, K., Stojilković, S, Torsello, A, Iida, T, Rojas, E, Catt, K, TORSELLO, ANTONIO BIAGIO, and Catt, K.

Abstract

In cultured pituitary gonadotrophs, gonadotropin-releasing hormone (GnRH) caused dose-dependent and biphasic increases in cytoplasmic calcium concentration ([Ca2+]i) and LH release. Both extra- and intracellular calcium pools participate in GnRH-induced elevation of [Ca2+]i and LH secretion. The spike phase of the [Ca2+]i response represents the primary signal derived predominantly from the rapid mobilization of intracellular Ca2+. In contrast, the prolonged phase of the Ca2+ signal depends exclusively on Ca2+ entry from the extracellular pool. The influx of Ca2+ occurs partially through dihydropyridine-sensitive calcium channels. Both [Ca2+]i and LH responses to increasing concentrations of GnRH occur over very similar time scales, suggesting that increasing degrees of receptor occupancy are transduced into amplitude-modulated Ca2+ responses, which in turn activate exocytosis in a linear manner. However, several lines of evidence indicated the complexity over the relationship between Ca2+ signaling and LH exocytosis. In contrast to [Ca2+]i measurements in cell suspension, single cell Ca2+ measurements revealed the existence of a more complicated pattern of Ca2+ response to GnRH, with a biphasic response to high agonist doses and prominent oscillatory responses to lower GnRH concentrations, with a log-linear correlation between GnRH dose and the frequency of Ca2+ spiking. In addition, analysis of the magnitudes of the [Ca2+]i and LH responses of gonadotrophs to a wide range of GnRH concentrations in the presence and absence of extracellular Ca2+, and to K+ and phorbol ester stimulation, showed non-linearity between these parameters with amplification of [Ca2+]i-mediated exocytosis. Studies on cell depleted of protein kinase C under conditions that did not change the LH pool suggested the participation of protein kinase C in this amplification, especially during the plateau phase of the secretory response to GnRH.

Published
1992

17. Steroids and tissue-specific modulation of galanin gene expression in the male rat reproductive system

Author

Torsello, A, Vrontakis, M, Schroedter, I, Vuille, J, Ikejiani, C, Friesen, H, TORSELLO, ANTONIO BIAGIO, Friesen, H., Torsello, A, Vrontakis, M, Schroedter, I, Vuille, J, Ikejiani, C, Friesen, H, TORSELLO, ANTONIO BIAGIO, and Friesen, H.

Abstract

Galanin is a neuropeptide widely distributed throughout the vertebrate neural and endocrine system. Galanin can influence pituitary hormone secretion, intestinal motility, and other biological activities. The precise physiological role of galanin is unknown. We studied the control of galanin gene expression in peripheral organs in the male rat using Northern blot and in situ hybridization techniques. In the adrenals and prostate, galanin mRNA was undetectable in the controls and did not change after the administration of dexamethasone (0.0001-10.0 mg/kg, ip) and diethylstilbestrol (0.1 mg/kg, ip). In the testis, thymus, seminal vesicles, medial basal hypothalamus, and colon, galanin message was detectable, but was not influenced by steroids. On the other hand, dexamethasone (0.5-10.0 mg/kg) was very effective in enhancing galanin expression in the vas deferens and epididymis (4- to 7-fold in the vas deferens), with a peak 6-9 h after the treatment. Diethylstilbestrol (0.1 mg/kg) stimulated galanin mRNA transcription only in the vas deferens (2- to 3-fold), with a peak 1-3 h after the treatment. Dihydrotestosterone treatment (0.2-0.4 mg/kg) was ineffective in all tissues examined. In the vas deferens and seminal vesicles, galanin mRNA has been localized at a cellular level by in situ hybridization. In these tissues only fibroblast-like cells contained the message. These data demonstrate that galanin is expressed in the male rat reproductive system and that steroid hormones participate in the control of galanin gene expression in a tissue- and hormone-specific fashion.

Published
1992

18. Na+,2Cl-,K+ cotransport system as a marker of antihypertensive activity of new torasemide derivatives

Author

Masereel, B, Ferrari, P, Ferrandi, M, Pirotte, B, Schynts, M, Parenti, P, Delarge, J, Delarge, J., PARENTI, PAOLO, Masereel, B, Ferrari, P, Ferrandi, M, Pirotte, B, Schynts, M, Parenti, P, Delarge, J, Delarge, J., and PARENTI, PAOLO

Abstract

A series of compounds related to torasemide, a loop diuretic, were synthesized and examined for their diuretic potency and inhibitory activity on the erythrocyte and renal medullary thick ascending limb vesicle Na+,2Cl-,K+ cotransport in Milan hypertensive (MHS) and normotensive (MNS) rat strains, where previous studies had demonstrated an alteration of the cotransport system genetically related to hypertension. From the results of the screening, structure-activity relationships were drawn and two compounds, JDL 961 and C 2921 were selected. Their IC50 on renal vesicle cotransport were similar in the two strains (JDL 961: MHS = 1.8 microM; MNS = 1.2 microM; C 2921: MHS = 4 microM; MNS = 3.8 microM), and were 4-8 times lower than those of torasemide (MHS = 13 microM; MNS = 31 microM, P less than 0.01) and 50-60 times lower than those of bumetanide (MHS = 145 microM; MNS = 206 microM, P less than 0.05) taken as reference compounds. Their ability to reduce the development rate of hypertension was tested both in MHS and in Okamoto spontaneously hypertensive rats (SHR) strain, in which cotransport alterations are opposite to those of MHS. Both torasemide derivatives (7.5 mg.kg-1 os per day) prevented development of hypertension in the two strains. The time course of this hypotensive activity was faster and the percentage of blood pressure fall greater in MHS (20-25%) than in SHR rats (12-15%), even though the absolute value of blood pressure fall was similar in MHS (JDL 961 = -17 mm Hg; C 2921 = -30 mm Hg) and SHR (JDL 961 = -25 mm Hg; C 2921 = -20 mm Hg). A superimposable effect of bumetanide was observed in the two strains, but at 8 times higher daily dose (60 mg.kg-1). These results suggest that new loop diuretics can be selected for their antihypertensive activity on the basis of their in vitro potency in inhibiting the Na+,2Cl-,K+.

Published
1992

19. Different neuronal types in transneuronally WGA-HRP-labeled premotor interneurons of the rat spinal cord

Author

Isabella Barajon, Giovanni Tredici, Giuliano Pizzini, L. Vizzotto, Barajon, I, Vizzotto, L, Pizzini, G, and Tredici, G

Subjects
genetic structures, Interneuron, Rats, Inbred Strain, Afferent Pathway, Wheat Germ Agglutinins, Central nervous system, Population, Wheat Germ Agglutinin-Horseradish Peroxidase Conjugate, Cell Count, Biology, Horseradish peroxidase, Lumbar enlargement, Behavioral Neuroscience, Interneurons, medicine, Animals, education, Horseradish Peroxidase, Motor Neurons, education.field_of_study, Afferent Pathways, Animal, musculoskeletal, neural, and ocular physiology, Muscles, fungi, Rats, Inbred Strains, Anatomy, Motor neuron, Spinal cord, Wheat germ agglutinin, Rats, medicine.anatomical_structure, nervous system, Spinal Cord, biology.protein, Rat, Muscle, Wheat Germ Agglutinin, Neuroscience
Abstract

Interneurons presynaptic to motoneurons were labeled by retrograde transneuronal transport of WGA-HRP. The tracer was injected either into the quadriceps muscles or into the posterior biceps muscles, thus labeling interneurons presynaptic to the quadriceps motoneurons (QINs) or interneurons presynaptic to posterior biceps motoneurons (PBINs). Statistical cluster analysis of area, perimeter, equivalent diameter and form factor of the labeled interneurons permitted the identification of 4 different types of premotor interneurons in the lumbar enlargement of the rat. Type I are small elongated interneurons which prevail in PBINs. Type II are medium-sized ellipsoidal cells prevailing in the QINs. Type 3 are small ellipsoidal neurons, slightly more frequent in PBINs. Type 4 is the smallest group and it is composed of large multipolar neurons. A different distribution of the 4 morphological neuronal types was found between the population of the QINs and the PBINs and in the laminae of ventral horn for each group.

Published
1990

20. 99mTc complexes of alpha,alpha-disubstituted, alpha-hydroxy carboxylic acids

Author

F, Colombo, M, Matarrese, F, Fazio, E, Deutsch, Colombo, F, Matarrese, M, Fazio, F, and Deutsch, E

Subjects
Rats, Inbred Strain, Animal, Malate, Urinary Bladder, Malates, Hydroxybutyrates, Rats, Inbred Strains, Organotechnetium Compounds, Kidney, Rats, Dogs, Drug Stability, Dog, Animals, Rat, Tissue Distribution, Female, Radionuclide Imaging, Organotechnetium Compound
Abstract

99mTc complexes of 2-ethyl-2-hydrobutyric acid, 2-hydroxyisobutyric acid and (+)- and (-)-citramalic acid are readily prepared in high yield and high purity by reduction of 99mTcO4- in the presence of excess ligand. The resulting agents are very stable in vitro, but can undergo some decomposition during chromatographic analysis unless appropriate precautions are taken. Biodistribution studies in rats and dogs show that these new 99mTc agents accumulate primarily in the kidney and urinary bladder.

Published
1990

21. The spinal terminals into the midbrain periaqueductal gray of the rat. A light and electron microscope study of the projections ascending via the ventro-lateral funiculus

Author

R, Bianchi, G, Tredici, M, Gioia, Bianchi, R, Tredici, G, and Gioia, M

Subjects
Nerve Endings, Nerve Ending, Male, Rats, Inbred Strain, Animal, Rats, Inbred Strains, Dendrites, Dendrite, Rats, Microscopy, Electron, Spinal Cord, Mesencephalon, Animals, Rat, Periaqueductal Gray, Horseradish Peroxidase
Abstract

Light and electron microscope studies of the terminal fields of the spinal afferents ascending in the ventrolateral quadrant of the spinal cord to the periaqueductal gray matter (PAG) were carried out using silver degeneration techniques and anterograde WGA-HRP transport. At all mesencephalic levels the terminal degeneration and the labelling of the spinal fibres to the PAG were fairly dense, mainly concentrated in the outer part of the annular ring. At the electron microscope, the spinal nerve terminals were found ending almost exclusively in the neuropil, impinging on small dendritic profiles. The majority of these synaptic contacts were of the asymmetrical type and contained a prevalence of round vesicles. This study provides an accurate representation of the terminal domain of the spino-PAG afferents and gives the conclusive anatomical evidence that the fibres ascending in the ventro-lateral funiculus of the spinal cord do not simply pass through the PAG, but actually terminate in it, synapsing in the neuropil.

Published
1990

22. Interactions between calcium and protein kinase C in the control of signaling and secretion in pituitary gonadotrophs

Author

Stojilković, S, Iida, T, Merelli, F, Torsello, A, Krsmanović, L, Catt, K, TORSELLO, ANTONIO BIAGIO, Catt, K., Stojilković, S, Iida, T, Merelli, F, Torsello, A, Krsmanović, L, Catt, K, TORSELLO, ANTONIO BIAGIO, and Catt, K.

Abstract

Single pituitary gonadotrophs exhibit episodes of spontaneous fluctuations in cytoplasmic calcium concentration [( Ca2+]i) due to entry through voltage-sensitive calcium channels (VSCC) and show prominent agonist-induced oscillations in [Ca2+]i that are generated by periodic release of intracellular Ca2+. Gonadotropin releasing hormone (GnRH) elicited three types of Ca2+ responses: at low doses, subthreshold, with an increase in basal [Ca2+]i; at intermediate doses, oscillatory, with dose-dependent modulation of spiking frequency; and at high doses, biphasic, without oscillations. Elevation of [Ca2+]i or activation of protein kinase C (PKC) did not influence the frequency of agonist-induced [Ca2+]i spikes but caused dose-dependent reductions in amplitude for all types of Ca2+ response. Stimulation of transient Ca2+ spikes by GnRH was followed by inhibition of the spontaneous fluctuations. GnRH also reduced the ability of high extracellular K+ to promote Ca2+ influx through VSCC. Activation of PKC by phorbol esters stimulated Ca2+ influx in quiescent cells but inhibited influx when VSCC were already activated, either spontaneously or by high K+. In contrast to their biphasic actions on [Ca2+]i, phorbol esters exerted only stimulatory actions on gonadotropin release, even when Ca2+ influx was concomitantly reduced. However, pituitary cells had to be primed with an appropriate [Ca2+]i level before exocytosis could be amplified by PKC. In PKC-depleted cells, all actions of phorbol esters on Ca2+ entry and amplitude modulation, and on LH release, were abolished. GnRH-induced LH secretion was also significantly reduced, especially the plateau phase of the response. These data indicate that Ca2+ and PKC serve as interacting signals during the cascade of cellular events triggered by agonist stimulation, in which Ca2+ turns cell responses on or off, and PKC amplifies the positive and negative effects of Ca2+

Published
1991

23. 99mTc complexes of alpha,alpha-disubstituted, alpha-hydroxy carboxylic acids

Author

Colombo, F, Matarrese, M, Fazio, F, Deutsch, E, Deutsch, E., FAZIO, FERRUCCIO, Colombo, F, Matarrese, M, Fazio, F, Deutsch, E, Deutsch, E., and FAZIO, FERRUCCIO

Abstract

99mTc complexes of 2-ethyl-2-hydrobutyric acid, 2-hydroxyisobutyric acid and (+)- and (-)-citramalic acid are readily prepared in high yield and high purity by reduction of 99mTcO4- in the presence of excess ligand. The resulting agents are very stable in vitro, but can undergo some decomposition during chromatographic analysis unless appropriate precautions are taken. Biodistribution studies in rats and dogs show that these new 99mTc agents accumulate primarily in the kidney and urinary bladder.

Published
1990

24. Na+/K+/Cl(-)-cotransporter mediated Rb+ fluxes in membrane vesicles from kidneys of normotensive and hypertensive rats

Author

Ferrandi, M, Salardi, S, Parenti, P, Ferrari, P, Bianchi, G, Braw, R, Karlish, S, PARENTI, PAOLO, Karlish, SJ, Ferrandi, M, Salardi, S, Parenti, P, Ferrari, P, Bianchi, G, Braw, R, Karlish, S, PARENTI, PAOLO, and Karlish, SJ

Abstract

This paper describes experiments to examine Rb+ fluxes via the Na+/K+/Cl- cotransporter in membrane vesicles from renal outer medulla of three strains of rat: (A) Wistar (B) Milan hypertensive (MHS) and normotensive (MNS), and (C) Sabra salt-sensitive hypertensive (SBH) and salt-resistant (SBN). Initially, Na(+)-dependent furosemide- or bumetanide-inhibited 86Rb+ fluxes were characterised using Wistar rat microsomes. The latter were partially purified on a metrizamide cushion, and assay conditions were optimized for use with microsomes from the other rats. The major result is that in microsomes from adult Milan hypertensive (MHS) rats the rate of the Na+/K+/Cl(-)-cotransporter mediated 86Rb flux at sub-saturating concentrations of Rb, appears to be significantly greater than in the normotensive (MNS) controls. The effect reflects an increased apparent Rb affinity of the cotransporter in MHS microsomes. There is no difference in maximal rate or in the apparent Na+ activation affinity of the 86Rb+ flux. In addition bumetanide appears to be a somewhat more effective inhibitor in MHS compared to MNS microsomes. The 86Rb+ flux result is compatible with a previous finding that in red cells, Na+/K+ -cotransporter mediated fluxes are increased in MHS compared to MNS. It supports the notion that the Na+/K+/Cl(-)-cotransporter in in both red cells and kidney is a genetic marker for hypertension. It is of interest that apparently more than one Na+ transport system is affected in MHS hypertensive kidneys (a) the Na+/K+/Cl- cotransporter in the thick ascending limb of Henle and (b) the Na+/H+ exchanger and/o a conductive Na(+)-pathway in brush-border membranes from proximal tubule. It is conceivable that in the hypertensive animals a common regulatory pathway (e.g., phosphorylation) or protein (e.g., cytoskeleton) is affected along the length of the nephron. In Sabra SBH and SBN rat microsomes, no difference was found for the 86Rb+ flux via the Na+/K+/Cl- cotransporter (or via a

Published
1990

25. The spinal terminals into the midbrain periaqueductal gray of the rat. A light and electron microscope study of the projections ascending via the ventro-lateral funiculus

Author

Bianchi, R, Tredici, G, Gioia, M, Gioia, M., TREDICI, GIOVANNI, Bianchi, R, Tredici, G, Gioia, M, Gioia, M., and TREDICI, GIOVANNI

Abstract

Light and electron microscope studies of the terminal fields of the spinal afferents ascending in the ventrolateral quadrant of the spinal cord to the periaqueductal gray matter (PAG) were carried out using silver degeneration techniques and anterograde WGA-HRP transport. At all mesencephalic levels the terminal degeneration and the labelling of the spinal fibres to the PAG were fairly dense, mainly concentrated in the outer part of the annular ring. At the electron microscope, the spinal nerve terminals were found ending almost exclusively in the neuropil, impinging on small dendritic profiles. The majority of these synaptic contacts were of the asymmetrical type and contained a prevalence of round vesicles. This study provides an accurate representation of the terminal domain of the spino-PAG afferents and gives the conclusive anatomical evidence that the fibres ascending in the ventro-lateral funiculus of the spinal cord do not simply pass through the PAG, but actually terminate in it, synapsing in the neuropil

Published
1990

26. Different neuronal types in transneuronally WGA-HRP-labeled premotor interneurons of the rat spinal cord

Author

Barajon, I, Vizzotto, L, Pizzini, G, Tredici, G, Barajon, I, Vizzotto, L, Pizzini, G, and Tredici, G

Abstract

Interneurons presynaptic to motoneurons were labeled by retrograde transneuronal transport of WGA-HRP. The tracer was injected either into the quadriceps muscles or into the posterior biceps muscles, thus labeling interneurons presynaptic to the quadriceps motoneurons (QINs) or interneurons presynaptic to posterior biceps motoneurons (PBINs). Statistical cluster analysis of area, perimeter, equivalent diameter and form factor of the labeled interneurons permitted the identification of 4 different types of premotor interneurons in the lumbar enlargement of the rat. Type I are small elongated interneurons which prevail in PBINs. Type II are medium-sized ellipsoidal cells prevailing in the QINs. Type 3 are small ellipsoidal neurons, slightly more frequent in PBINs. Type 4 is the smallest group and it is composed of large multipolar neurons. A different distribution of the 4 morphological neuronal types was found between the population of the QINs and the PBINs and in the laminae of ventral horn for each group

Published
1990

27. Lens redox fluorometry: Pyridine nucleotide fluorescence and analysis of diabetic lens

Author

Joel M. Krauss, Ronald A. Laing, Hong Ming Cheng, Kenneth R. Kenyon, Kazuo Tsubota, Stefano Miglior, Tsubota, K, Krauss, J, Kenyon, K, Laing, R, Miglior, S, and Cheng, H

Subjects
Rats, Inbred Strain, Rabbit, Fluorescence, Fluorescence spectroscopy, Diabetes Mellitus, Experimental, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Polyol pathway, In vivo, Fluorometer, Lens, Crystalline, medicine, Animals, Fluorometry, Aldose reductase, Animal, Chemistry, Rats, Inbred Strains, NAD, Aldose reductase inhibitor, Sensory Systems, Rats, Ophthalmology, Biochemistry, Biophysics, Rat, Sorbinil, Rabbits, Oxidation-Reduction, medicine.drug
Abstract

We performed both ex vivo and in vivo fluorometric analyses of pyridine nucleotides (PN) in rabbit and rat lenses. Rabbit lens PN fluorescence (99% NADH) was found to have an excitation maximum at 366 nm and an emission maximum at 462 nm (366:462). The only other fluorescent chromophore in that region of the spectrum has excitation and emission peaks at 328 and 460 nm, respectively. Anaerobic glycolysis in the lens was stimulated by KCN, a known inhibitor of mitochondrial respiration, after which a time-study of fluorescence intensities was performed. Over the course of a 3.5 hr period following treatment with KCN, the PN signal showed a statistically significant increase relative to that in the control lenses (those treated with KCl). while the 328:460 signal (which may be due to some protein involved in energy transfer with the PN) had a significantly greater decrease. We also found that fluorescence intensity of NADH in solution is linearly proportional to physiologic-range concentration. Moreover, there was a close correlation between fluorescence intensity of rat lens PN as measured on a specular microscope-coupled redox fluorometer capable of in vivo use, and the lens PN levels as determined by the analytical cycling assay technique. This fluorometer was then employed to assess the redox state in rats with streptozotocin-induced diabetes. The normalized ratio of PN to flavoproteins (Fp) in the lens epithelium increased from 0.96 +/- 0.12 in the normal state to 1.48 +/- 0.30 2 weeks after diabetes induction. In contrast, the ratio in the diabetic lens treated with an aldose reductase inhibitor, sorbinil, did not increase. The increase in the PN:Fp ratio therefore reflects activation of the polyol pathway and its associated metabolic activities, which results in an increase in the NADH:NAD ratio in the diabetic rat lenses. Our results indicate that the non-invasive, real-time method of redox fluorometry may be useful in the early detection and evaluation of cataracts and other disorders in lens metabolism, long before opacities occur. It can be used to monitor the disease process and evaluate the efficacy of such drugs as aldose reductase inhibitors on a biochemical level.

Published
1989
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28. Excitatory Effect of Converting Enzyme Inhibitors on Efferent Sympathetic Postganglionic Nerve Activity to the Kidney in the Rat

Author

G. Recordati, D. Cerati, P. Gerometta, Simonetta Genovesi, R. Di Cintio, Recordati, G, Genovesi, S, Cerati, D, Di Cintio, R, and Gerometta, P

Subjects
Male, medicine.medical_specialty, Captopril, Baroreceptor, Rats, Inbred Strain, Efferent, Angiotensin-Converting Enzyme Inhibitors, Kidney, Efferent Pathways, Efferent Pathway, chemistry.chemical_compound, Adrenergic Fiber, Internal medicine, Heart rate, medicine, Animals, Hemodynamic, Teprotide, Evoked Potentials, Animal, business.industry, Hemodynamics, Angiotensin-Converting Enzyme Inhibitor, Rats, Inbred Strains, General Medicine, Spinal cord, Rats, Autonomic nervous system, medicine.anatomical_structure, Endocrinology, chemistry, Rat, Autonomic Fibers, Postganglionic, Evoked Potential, Adrenergic Fibers, business
Abstract

1. Experiments were designed to evaluate the effect of converting enzyme inhibitors on autonomic nervous system function in the rat. 2. Arterial blood pressure, heart rate, efferent postganglionic sympathetic activity and afferent nerve activity from the right renal nerves were recorded in anaesthetized, spontaneously breathing, non diuretic rats, either with an intact spinal cord or with a spinal cord transected at the T6 level, before, during and after intravenous injections of 0.5–1.0 mg/kg of teprotide or captopril. 3. After injection of drugs, efferent sympathetic nerve activity markedly increased and reached its peak value 4 min later, both in rats with an intact spinal cord (101 ± 21% mean ± se, above the control discharge) and with a spinal cord transected at the T6 level (166 ± 41%, above the control). 4. Afferent activity from the renal nerve, on the other hand, did not consistently change during converting enzyme blockade. 5. The results indicate that the efferent sympathetic excitation cannot be due either to a baroreceptor or to a renorenal reflex. This excitation might be responsible, at least in part, for the increase in renin secretion which follows the blockade of angiotensin-converting enzyme.

Published
1981
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30. Interference of the new antiinflammatory compound flunoxaprofen with eicosanoid formation in various biological systems

Author

Berti, F, Galli, G, Omini, C, Rossoni, G, Brunelli, G, Daffonchio, L, Viganò, T, Magni, F, Crivellari, M, Forgione, A, Forgione, A., MAGNI, FULVIO, Berti, F, Galli, G, Omini, C, Rossoni, G, Brunelli, G, Daffonchio, L, Viganò, T, Magni, F, Crivellari, M, Forgione, A, Forgione, A., and MAGNI, FULVIO

Abstract

S-(+)-2-(4-Fluorophenyl)-alpha-methyl-5-benzoxazolacetic acid (flunoxaprofen, Priaxim is a new antiinflammatory compound, which in various biological systems interferes with the generation and release of arachidonic acid metabolites of the cyclo-oxygenase pathways without affecting the formation of 5- and 12-lipoxygenase products. Flunoxaprofen reduces the concentration of thromboxane (TX)B2 (ED50 = 35.4 mg/kg p.o.) and prostaglandin (PG)E2-like activity (ED50 = 39.9 mg/kg p.o.) in the inflammatory exudate of rats 8 h after implantation of sponges soaked with carrageenan, whereas the concentration of leukotriene (LT)B4 remains in the range of that of the untreated animals (3.1 ng/ml). Flunoxaprofen inhibits cell infiltration in the exudate and this suggests that LTB4 does not initiate cell recruitment but may represent a mechanism for amplifying the inflammatory response. Using human platelets challenged with collagen, flunoxaprofen only at higher concentration (10(-4) mol/l) reduces TXB2 formation without altering generation of 12-hydroxy-5,8,10,14-eicosatetraenoic acid. This suggests a low capacity of flunoxaprofen of affecting platelet aggregation regulated by arachidonic acid metabolites. Flunoxaprofen prevents pulmonary changes due to secondary release of TXA2 in the guinea-pig. In fact this drug prevents changes due to immunological reaction and antagonizes bronchoconstriction due to exogenous administration of histamine and LTC4.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1987

31. Renorenal reflexes in the rat elicited upon stimulation of renal chemoreceptors

Author

Recordati, G, Genovesi, S, Cerati, D, Cerati, D., GENOVESI, SIMONETTA CARLA, Recordati, G, Genovesi, S, Cerati, D, Cerati, D., and GENOVESI, SIMONETTA CARLA

Abstract

The effects of renal ischemia and backflow of non-diuretic urine into the renal pelvis on renal efferent sympathetic postganglionic nerve activity, femoral arterial pressure and heart rate were studied to verify whether stimulation of renal chemoreceptors elicits autonomic reflexes. In rats with intact spinal cord or spinal cord sectioned at the T6 level a brief activation of renal chemoreceptors produced excitatory ipsilateral and contralateral renorenal reflexes, whereas it only slightly and insignificantly altered arterial pressure and heart rate. These results indicate that stimulation of renal chemoreceptors elicits renorenal excitatory reflexes which might be integrated both at spinal and supraspinal levels.

Published
1982

32. Renal chemoreceptors

Author

Recordati, G, Moss, N, Genovesi, S, Rogenes, P, Rogenes, P., GENOVESI, SIMONETTA CARLA, Recordati, G, Moss, N, Genovesi, S, Rogenes, P, Rogenes, P., and GENOVESI, SIMONETTA CARLA

Abstract

A study of the renal receptors and types of stimuli which give origin to supraspinal and spinal-mediated autonomic reflexes is presented. Multiunit and single unit recordings from the afferent renal nerves of male Sprague-Dawley rats have revealed two groups of renal chemosensitive receptors (chemoreceptors). These we have called renal R1 and R2 "chemoceptive" receptors. R1 receptors do not have a resting discharge but are activated after 38.7 +/- 3.3 (S.E) sec (n = 40) of complete renal ischemia (occlusion of the renal artery). Other activating stimuli are associated with a marked impairment in renal blood flow (prolonged occlusion of the renal vein and the hypotension of systemic asphyxia or hemorrhage). Their discharge is characterized by trains of impulses which cease abruptly upon re-entry of blood into the kidney. They are not responsive to increases or decreases in renal perfusion pressure or to increases in renal venous or ureteral pressure. In contrast, R2 receptors have a resting discharge and respond vigorously to backflow of normal urine (nondiuretic) into the renal pelvis. The results of the backflow into the pelvis of different test solutions (diuretic and nondiuretic urine, 1 M urea, 1 M mannitol and solutions of NaCl and KCl) indicate that this response is dependent upon the composition of the fluid bathing the renal pelvis rather than the increase in pelvic pressure or pelvic distension. The resting discharge rate is highest in nondiuretic conditions and declines substantially after diuresis is induced by extracellular volume expansion. R2 receptors are also activated by renal ischemia produced by clamping the renal artery. It is concluded that these two groups of afferent sensory units are renal chemosensitive receptors, (chemoreceptors) which respond to the chemical environment of renal interstitium.

Published
1981

33. Excitatory effect of converting enzyme inhibitors on efferent sympathetic postganglionic nerve activity to the kidney in the rat

Author

Recordati, G, Genovesi, S, Cerati, D, Di Cintio, R, Gerometta, P, Gerometta, P., GENOVESI, SIMONETTA CARLA, Recordati, G, Genovesi, S, Cerati, D, Di Cintio, R, Gerometta, P, Gerometta, P., and GENOVESI, SIMONETTA CARLA

Abstract

1. Experiments were designed to evaluate the effect of converting enzyme inhibitors on autonomic nervous system function in the rat. 2. Arterial blood pressure, heart rate, efferent postganglionic sympathetic activity and afferent nerve activity from the right renal nerves were recorded in anaesthetized, spontaneously breathing, non diuretic rats, either with an intact spinal cord or with a spinal cord transected at the T6 level, before, during and after intravenous injections of 0.5--1.0 mg/kg of teprotide or captopril. 3. After injection of drugs, efferent sympathetic nerve activity markedly increased and reached its peak value 4 min later, both in rats with an intact spinal cord (101 +/- 21% mean +/- SE, above the control discharge) and with a spinal cord transected at the T6 level (166 +/- 41%, above the control). 4. Afferent activity from the renal nerve, on the other hand, did not consistently change during converting enzyme blockade. 5. The results indicate that the efferent sympathetic excitation cannot be due either to a baroreceptor or to a renorenal reflex. This excitation might be responsible, at least in part, for the increase in renin secretion which follows the blockade of angiotensin-converting enzyme.

Published
1981

34. Role of the renal nerves in the natriuretic response to vasopressin infusion

Author

Genovesi, S, Protasoni, G, Golin, R, Stella, A, Zanchetti, A, GENOVESI, SIMONETTA CARLA, STELLA, ANDREA, Zanchetti, A., Genovesi, S, Protasoni, G, Golin, R, Stella, A, Zanchetti, A, GENOVESI, SIMONETTA CARLA, STELLA, ANDREA, and Zanchetti, A.

Abstract

The present study was designed to determine whether renal nerves influence the natriuretic response to an infusion of vasopressin. Experiments were performed on anaesthetized rats in which the response to vasopressin of the innervated kidney was compared with that of the contralateral surgically denervated kidney. During the vasopressin infusion the natriuretic effect was evident in both kidneys and was proportionally greater in the innervated kidney than in the denervated one. Efferent renal nerve activity, recorded in three additional animals, decreased during the vasopressin infusion. Our data demonstrate that the natriuretic response of the innervated kidney is larger than that of the denervated kidney, probably because of an associated decrease in efferent renal nerve activity.

Published
1989

37. Metabolic and kinetic considerations in the use of [125I]HIPDM for quantitative measurement of regional cerebral blood flow

Author

Lucignani, G, Nehlig, A, Blasberg, R, Patlak, C, Anderson, L, Fieschi, C, Fazio, F, Sokoloff, L, Sokoloff, L., FAZIO, FERRUCCIO, Lucignani, G, Nehlig, A, Blasberg, R, Patlak, C, Anderson, L, Fieschi, C, Fazio, F, Sokoloff, L, Sokoloff, L., and FAZIO, FERRUCCIO

Abstract

The metabolic degradation and the kinetics of the cerebral uptake of N,N,N'-trimethyl-N'-(2-hydroxy-3-methyl-5-[125I]iodobenzyl)-1, 3-propanediamine ([125I]HIPDM) have been studied in conscious, adult male Sprague-Dawley rats to determine its suitability as a tracer for the quantitative measurement of regional CBF (rCBF). rCBF was calculated by the indicator fractionation and the tissue equilibration methods in experiments of different durations up to 1 h. The values of rCBF obtained with [125I]HIPDM were compared with those obtained in concurrent measurements with [14C]iodoantipyrine in the same animals. Results of the experiments demonstrate that [125I]HIPDM is an inadequate tracer for use with the indicator fractionation method and that any method that employs [125I]HIPDM for the determination of rCBF must take into account its metabolic degradation, diffusion limitations, and bidirectional flux across the blood-brain barrier. With the tissue equilibration method, consistent determinations of rCBF may be possible with [125I]HIPDM by measurement of the time course of its concentration in arterial blood, corrected for the presence of 125I-labeled metabolic products, and its concentration in the brain at any time up to 1 h after its administration. The method may be adapted to measure rCBF in humans by means of single-photon emission tomography with [123I]HIPDM.

Published
1985

38. Cholinergic agonist and antagonist drugs modulate the growth hormone response to growth hormone-releasing hormone in the rat: evidence for mediation by somatostatin

Author

Locatelli, V, Torsello, A, Redaelli, M, Ghigo, E, Massare, F, Müller, E, LOCATELLI, VITTORIO, TORSELLO, ANTONIO BIAGIO, Müller, E., Locatelli, V, Torsello, A, Redaelli, M, Ghigo, E, Massare, F, Müller, E, LOCATELLI, VITTORIO, TORSELLO, ANTONIO BIAGIO, and Müller, E.

Abstract

Recently, data have been presented showing that muscarinic cholinergic agonists or antagonists can modulate, in opposite ways, GH-releasing hormone GHRH)-induced GH release in man. The aim of the present study was, first, to confirm these findings in the rat and, secondly, if confirmed, to investigate the mechanism(s) subserving the effect of cholinergic drugs. In adult male rats bearing chronic indwelling atrial cannulae, pretreatment with the cholinergic antagonists pirenzepine (0.5 mg/kg, i.v.) or atropine (0.5 mg/kg, i.v.) significantly reduced the rise in plasma GH induced by GHRH (2 micrograms/kg, i.v.), while pretreatment with the cholinergic agonist pilocarpine (3 mg/kg, i.v.) potentiated it. In rats with hypothalamic somatostatin (SRIF) depletion, i.e. rats with anterolateral deafferentation of the mediobasal hypothalamus or rats treated with cysteamine, the modulatory action of cholinergic drugs on the neuroendocrine effect of GHRH was completely lacking. In these two experimental models, an antiserum raised against SRIF failed to elicit a rise in plasma GH and measurement of hypothalamic SRIF content revealed a clear-cut reduction of the neuropeptide. Atropine (1 mumol/l) and pilocarpine (1 mumol/l), added to pituitary cells in vitro, failed to alter GHRH-induced GH release. The present results indicate that muscarinic cholinergic agonists and antagonists modulate GHRH-induced GH release in the rat and suggest that the effect of cholinergic modulation takes place through SRIF.

Published
1986

39. A renal abnormality in the Milan hypertensive strain of rats and in humans predisposed to essential hypertension

Author

Bianchi, G, Ferrari, P, Salvati, P, Salardi, S, Parenti, P, Cusi, D, Guidi, E, Guidi, E., PARENTI, PAOLO, Bianchi, G, Ferrari, P, Salvati, P, Salardi, S, Parenti, P, Cusi, D, Guidi, E, Guidi, E., and PARENTI, PAOLO

Abstract

Many similarities in kidney-function abnormalities were found between hypertensive rats of the Milan strain (MHS) and young normotensive human subjects with hypertensive parents, compared with the appropriate controls. These similarities included an increased glomerular filtration rate, increased pressor effect of the kidney after transplantation, increased 24-h urinary output and lower plasma renin activity and urinary kallikrein. The isolated MHS kidney perfused in vitro with an artificial medium had a higher glomerular filtration rate, a higher urinary output, higher tubular sodium reabsorption and higher oxygen consumption than the kidney of control Milan normotensive rats (MNS). Further, reogenic sodium transport across brush border vesicles isolated from proximal tubular cells is faster in MHS than in MNS. Erythrocytes and proximal tubular cells of MHS have a lower volume and sodium content than those of MNS, while sodium transport is faster and the Ca2+-ATPase at Vmax is lower. This indicates that the 'genetic' cellular abnormality responsible for the renal-function abnormality and the hypertension is also present in erythrocytes. Thus these cells may be used to study the genetic cellular mechanisms of hypertension. Experiments with bone marrow transplantation and with F2 hybrids obtained by crossing the F1 (MHS X MNS) hybrids showed that the MHS erythrocyte abnormalities are genetically determined within the stem cells and are genetically associated with the hypertension. Since, in human hypertensives, there was a correlation between abnormal erythrocyte sodium transport and renal function, it is proposed that erythrocytes may be used in studying the cellular molecular mechanisms of hypertension.

Published
1986

40. Involvement of the somatostatin and cholinergic systems in the mechanism of growth hormone autofeedback regulation in the rat

Author

Torsello, A, Panzeri, G, Cermenati, P, Caroleo, M, Ghigo, E, Camanni, F, Müller, E, Locatelli, V, TORSELLO, ANTONIO BIAGIO, LOCATELLI, VITTORIO, Torsello, A, Panzeri, G, Cermenati, P, Caroleo, M, Ghigo, E, Camanni, F, Müller, E, Locatelli, V, TORSELLO, ANTONIO BIAGIO, and LOCATELLI, VITTORIO

Abstract

The involvement of the cholinergic system in GH secretion has recently acquired increasing importance. Data have been presented suggesting that in rats the effect of cholinergic modulation on GH secretion takes place through inhibition or stimulation of hypothalamic somatostatin (SRIF) release. To investigate further the significance of cholinergic-SRIF link and its role in the regulation of GH secretion, the action of cholinergic agonist and antagonist drugs in the GH short-loop feedback mechanism mediated by SRIF was investigated. Intracerebroventricular (i.c.v.) infusion of 0.2 or 2.0 micrograms GH/rat into the lateral brain ventricle of adult male rats induced a significant reduction in the GH-releasing hormone (GHRH; 2 micrograms/kg, i.v.)-induced peak GH rise, but only the 2.0 micrograms dose reduced also the GH-integrated area after administration of GHRH. This effect was absent after central administration of 20.0 micrograms GH/rat, due probably to leakage of some GH from the cerebral ventricle into the systemic circulation. Pretreatment with cysteamine (300 mg/kg, s.c.), a known depletor of hypothalamic SRIF, or with anti-SRIF serum (0.5 ml/rat) completely counteracted the lessening of the GH response to GHRH induced by 2.0 micrograms GH injected i.c.v. Similarly, pretreatment with the cholinergic agonist pilocarpine (3 mg/kg, i.v.) completely antagonized the inhibitory effect of central infusion of GH on the GHRH-induced GH response. Atropine (1.0 mg/kg, i.v.), a muscarinic cholinergic antagonist, strikingly inhibited the GHRH-induced GH rise, but when given in combination with i.c.v. infusion of GH there was no additive inhibitory effect.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1988

41. Localization of synapsin I at the frog neuromuscular junction

Author

Valtorta, F, Villa, A, Jahn, R, De Camilli, P, Greengard, P, Ceccarelli, B, Ceccarelli, B., VILLA, ANTONELLO, Valtorta, F, Villa, A, Jahn, R, De Camilli, P, Greengard, P, Ceccarelli, B, Ceccarelli, B., and VILLA, ANTONELLO

Abstract

We report here the results of immunocytochemical and biochemical studies on the localization of synapsin I, a nerve terminal--specific phosphoprotein, at the frog neuromuscular junction. Our results show that in this in situ synapse synapsin I is concentrated in the presynaptic compartment, where it appears to be associated with the synaptic vesicle membrane. Double immunoprecipitated synapsin I from homogenates of frog cutaneous pectoris muscles could be phosphorylated by the catalytic subunit of cyclic adenosine 5'-monophosphate-dependent protein kinase after gel electrophoresis and blotting onto nitrocellulose and could be subsequently identified by an immunoperoxidase technique. Experiments carried out in frog brain preparations indicate that frog synapsin I, like the mammalian protein, can be phosphorylated at different sites by exogenously added catalytic subunit of cyclic adenosine 5'-monophosphate-dependent protein kinase and Ca2+/calmodulin-dependent protein kinase II prepared from mammalian sources. The phosphorylation sites of frog synapsin I, as judged by phosphopeptide mapping, are somewhat different from those of mammalian synapsin I. The study of synapsin I and of the regulation of its state of phosphorylation at the neuromuscular junction may provide important information on its role in synaptic function, since at the present time this is one of the few systems in which a correlation among biochemical, immunocytochemical and electrophysiological results is possible.

Published
1988

42. Lens redox fluorometry: pyridine nucleotide fluorescence and analysis of diabetic lens

Author

Tsubota, K, Krauss, J, Kenyon, K, Laing, R, Miglior, S, Cheng, H, Cheng, H., MIGLIOR, STEFANO, Tsubota, K, Krauss, J, Kenyon, K, Laing, R, Miglior, S, Cheng, H, Cheng, H., and MIGLIOR, STEFANO

Abstract

We performed both ex vivo and in vivo fluorometric analyses of pyridine nucleotides (PN) in rabbit and rat lenses. Rabbit lens PN fluorescence (99% NADH) was found to have an excitation maximum at 366 nm and an emission maximum at 462 nm (366:462). The only other fluorescent chromophore in that region of the spectrum has excitation and emission peaks at 328 and 460 nm, respectively. Anaerobic glycolysis in the lens was stimulated by KCN, a known inhibitor of mitochondrial respiration, after which a time-study of fluorescence intensities was performed. Over the course of a 3.5 hr period following treatment with KCN, the PN signal showed a statistically significant increase relative to that in the control lenses (those treated with KCl). while the 328:460 signal (which may be due to some protein involved in energy transfer with the PN) had a significantly greater decrease. We also found that fluorescence intensity of NADH in solution is linearly proportional to physiologic-range concentration. Moreover, there was a close correlation between fluorescence intensity of rat lens PN as measured on a specular microscope-coupled redox fluorometer capable of in vivo use, and the lens PN levels as determined by the analytical cycling assay technique. This fluorometer was then employed to assess the redox state in rats with streptozotocin-induced diabetes. The normalized ratio of PN to flavoproteins (Fp) in the lens epithelium increased from 0.96 +/- 0.12 in the normal state to 1.48 +/- 0.30 2 weeks after diabetes induction. In contrast, the ratio in the diabetic lens treated with an aldose reductase inhibitor, sorbinil, did not increase. The increase in the PN:Fp ratio therefore reflects activation of the polyol pathway and its associated metabolic activities, which results in an increase in the NADH:NAD ratio in the diabetic rat lenses. Our results indicate that the non-invasive, real-time method of redox fluorometry may be useful in the early detection and evaluation of cata

Published
1989

43. 31P NMR studies of the diabetic lens

Author

González, R, Miglior, S, Von Saltza, I, Buckley, L, Neuringer, L, Cheng, H, Cheng, H., MIGLIOR, STEFANO, González, R, Miglior, S, Von Saltza, I, Buckley, L, Neuringer, L, Cheng, H, Cheng, H., and MIGLIOR, STEFANO

Abstract

Phosphorus-31 (31P) nuclear magnetic resonance (NMR) spectroscopic analyses of the crystalline lens from the experimental diabetic rat were performed. Qualitative and quantitative alterations in the phosphorus-31 NMR metabolic profile were observed over the course of 3 weeks after the induction of diabetes mellitus. Most striking was the appearance of two new, as yet unidentified, metabolites. These metabolites which resonate at 6.6 and 5.8 ppm were not detected in the normal lens. Compared to the normal lens, glycerol-3-phosphate (G3P) underwent an eightfold increase in concentration and phosphorylcholine decreased to one-third its initial level. The phosphodiesters, glycerophosphorylcholine (GPC) and glycerophosphorylethanolamine (GPE), decreased to barely detectable levels. Oral treatment of the diabetic animal with an aldose reductase inhibitor resulted in the preservation of an essentially normal lens 31P NMR spectrum. Except for the changes observed in glycerol-3-phosphate, these alterations have not been previously reported and raise new questions about the metabolic consequences of diabetes mellitus and the dependence of these alterations on the action of a single enzyme, aldose reductase

Published
1988

44. Distribution of the cortico-spinal fibres in the cervical and lumbar enlargements of the rat spinal cord

Author

Gemma, M, Perego, G, Pizzini, G, Tredici, G, GEMMA, MARTA, TREDICI, GIOVANNI, Gemma, M, Perego, G, Pizzini, G, Tredici, G, GEMMA, MARTA, and TREDICI, GIOVANNI

Abstract

We examined the distribution pattern of the corticospinal fibres in cervical and lumbar enlargements of the rat spinal cord with the Fink-Heimer silver impregnation method, after extensive cortical ablation. Corticospinal fibres are bilateral and run in the lateral and anterior funiculi. The distribution at the cervical and lumbar levels does not differ. The main area of termination are: 1) the lateral part of the ventral horn basis; 2) an area surrounding the motoneurons group posteriorly. At the electron microscope we were unable to find degenerating boutons of the corticospinal projections contacting HRP labelled motoneurons retrogradely. This indicates that at both levels few monosynaptic corticospinal fibres or none at all end on the motoneurons. Our study does not support the suggestion of differences in the termination pattern of the corticospinal tract of the rat between cervical and lumbar enlargements made on the basis of electrophysiological studies

Published
1987

45. Blood-nerve barrier of endoneural vessels in experimentally-induced hypothyroidism in rats

Author

Cavaletti, G, Barajon, I, Petruccioli, M, Tredici, G, CAVALETTI, GUIDO ANGELO, TREDICI, GIOVANNI, Cavaletti, G, Barajon, I, Petruccioli, M, Tredici, G, CAVALETTI, GUIDO ANGELO, and TREDICI, GIOVANNI

Abstract

Hypothyroidism may cause peripheral nerve damage, even if the pathophysiology of these changes is still unclear. It has been suggested by some that an increased vascular permeability is involved in hypothyroidism, while others have suggested a "compressive" mechanism caused by mucinous material deposited in the endoneurium. We have studied histologically the endoneurium and evaluated endoneural-vessel permeability in sciatic nerve by means of the leakage of horseradish peroxidase (HRP) in pharmacologically-induced hypothyroidism in rats. We did not find any substantial differences between the hypothyroid group of animals and the controls with respect to endoneural-vessel permeability. In particular, no macromolecular deposits were present in the extracellular space of the endoneurium in either the treated or the control rats. We therefore believe that a "vascular" hypothesis is unlikely for nerve involvement during hypothyroidism, nor was the "compressive" hypothesis supported by our histological findings

Published
1989

47. Cholinergic agonist and antagonist drugs modulate the growth hormone response to growth hormone-releasing hormone in the rat: evidence for mediation by somatostatin

Author

Redaelli M, E. E. Müller, Ezio Ghigo, Massare F, Locatelli, Antonio Torsello, Locatelli, V, Torsello, A, Redaelli, M, Ghigo, E, Massare, F, and Müller, E

Subjects
Male, Atropine, medicine.medical_specialty, Rats, Inbred Strain, Afferent Pathway, Endocrinology, Diabetes and Metabolism, Cysteamine, Hypothalamus, Neuropeptide, Hypothalamus, Middle, In Vitro Techniques, Biology, Peptide hormone, Growth Hormone-Releasing Hormone, Endocrinology, Internal medicine, medicine, Hypothalamu, Animals, BIO/14 - FARMACOLOGIA, Afferent Pathways, Animal, Parasympatholytic, Pilocarpine, Parasympatholytics, Rats, Inbred Strains, Pirenzepine, Growth hormone–releasing hormone, Rats, Somatostatin, Parasympathomimetics, Hormone receptor, Growth Hormone, Parasympathomimetic, Cholinergic, Rat, medicine.drug
Abstract

Recently, data have been presented showing that muscarinic cholinergic agonists or antagonists can modulate, in opposite ways, GH-releasing hormone (GHRH)-induced GH release in man. The aim of the present study was, first, to confirm these findings in the rat and, secondly, if confirmed, to investigate the mechanism(s) subserving the effect of cholinergic drugs. In adult male rats bearing chronic indwelling atrial cannulae, pretreatment with the cholinergic antagonists pirenzepine (0·5 mg/kg, i.v.) or atropine (0·5 mg/kg, i.v.) significantly reduced the rise in plasma GH induced by GHRH (2 μg/kg, i.v.), while pretreatment with the cholinergic agonist pilocarpine (3 mg/kg, i.v.) potentiated it. In rats with hypothalamic somatostatin (SRIF) depletion, i.e. rats with anterolateral deafferentation of the mediobasal hypothalamus or rats treated with cysteamine, the modulatory action of cholinergic drugs on the neuroendocrine effect of GHRH was completely lacking. In these two experimental models, an antiserum raised against SRIF failed to elicit a rise in plasma GH and measurement of hypothalamic SRIF content revealed a clear-cut reduction of the neuropeptide. Atropine (1 μmol/l) and pilocarpine (1 μmol/l), added to pituitary cells in vitro, failed to alter GHRH-induced GH release. The present results indicate that muscarinic cholinergic agonists and antagonists modulate GHRH-induced GH release in the rat and suggest that the effect of cholinergic modulation takes place through SRIF. J. Endocr. (1986) 111, 271–278

Published
1986

48. Metabolic and kinetic considerations in the use of [125I]HIPDM for quantitative measurement of regional cerebral blood flow

Author

Louis Sokoloff, Anderson L, Giovanni Lucignani, C. Fieschi, Clifford S. Patlak, Ronald G. Blasberg, Astrid Nehlig, Ferruccio Fazio, Lucignani, G, Nehlig, A, Blasberg, R, Patlak, C, Anderson, L, Fieschi, C, Fazio, F, and Sokoloff, L

Subjects
Male, Adult male, Rats, Inbred Strain, Equilibration method, Iodine Radioisotopes, Iodine Radioisotope, Nuclear magnetic resonance, TRACER, Single Photon Emission Tomography, Animals, Kinetic, business.industry, Iodobenzenes, Animal, Brain, Rats, Inbred Strains, Biological Transport, Blood flow, Cerebrovascular Circulation, Rats, Kinetics, Neurology, Cerebral blood flow, Blood-Brain Barrier, Iodobenzene, Rat, Neurology (clinical), Cardiology and Cardiovascular Medicine, Nuclear medicine, business, Mathematics, Mathematic, Tomography, Emission-Computed
Abstract

The metabolic degradation and the kinetics of the cerebral uptake of N, N, N'-trimethyl- N'-(2-hydroxy-3-methyl- 5-[125I]iodobenzyl)-1, 3-propanediamine ([125I]HIPDM) have been studied in conscious, adult male Sprague-Dawley rats to determine its suitability as a tracer for the quantitative measurement of regional CBF (rCBF). rCBF was calculated by the indicator fractionation and the tissue equilibration methods in experiments of different durations up to 1 h. The values of rCBF obtained with [125I]HIPDM were compared with those obtained in concurrent measurements with [14C]iodoantipyrine in the same animals. Results of the experiments demonstrate that [125I]HIPDM is an inadequate tracer for use with the indicator fractionation method and that any method that employs [125I]HIPDM for the determination of rCBF must take into account its metabolic degradation, diffusion limitations, and bidirectional flux across the blood-brain barrier. With the tissue equilibration method, consistent determinations of rCBF may be possible with [125I]HIPDM by measurement of the time course of its concentration in arterial blood, corrected for the presence of 125I-labeled metabolic products, and its concentration in the brain at any time up to 1 h after its administration. The method may be adapted to measure rCBF in humans by means of single-photon emission tomography with [123I]HIPDM.

Published
1985

49. Stimulating effect of converting enzyme inhibitors on the renal efferent post-ganglionic sympathetic nervous activity in the rat

Author

GENOVESI, SIMONETTA CARLA, Cerati, D, Di Cintio, R, Gerometta, P, Robatto, F, Recordati, G., Genovesi, S, Cerati, D, Di Cintio, R, Gerometta, P, Robatto, F, and Recordati, G

Subjects
Efferent Pathway, Male, Sympathetic Nervous System, Rats, Inbred Strain, Animal, Heart Rate, Neural Conduction, Rat, Autonomic Fibers, Postganglionic, Oligopeptide, Teprotide, Kidney
Published
1982

50. Distribution of the cortico-spinal fibres in the cervical and lumbar enlargements of the rat spinal cord

Author

Marco Gemma, Perego, G. B., Pizzini, G., Tredici, G., Gemma, M, Perego, G, Pizzini, G, and Tredici, G

Subjects
Decerebrate State, Staining and Labeling, Rats, Inbred Strain, Animal, Rats, Inbred Strains, Synapse, Axonal Transport, Rats, Microscopy, Electron, Spinal Cord, Synapses, Nerve Degeneration, Animals, Rat, Horseradish Peroxidase
Abstract

We examined the distribution pattern of the corticospinal fibres in cervical and lumbar enlargements of the rat spinal cord with the Fink-Heimer silver impregnation method, after extensive cortical ablation. Corticospinal fibres are bilateral and run in the lateral and anterior funiculi. The distribution at the cervical and lumbar levels does not differ. The main area of termination are: 1) the lateral part of the ventral horn basis; 2) an area surrounding the motoneurons group posteriorly. At the electron microscope we were unable to find degenerating boutons of the corticospinal projections contacting HRP labelled motoneurons retrogradely. This indicates that at both levels few monosynaptic corticospinal fibres or none at all end on the motoneurons. Our study does not support the suggestion of differences in the termination pattern of the corticospinal tract of the rat between cervical and lumbar enlargements made on the basis of electrophysiological studies.

Published
1987

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