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251. Development of a solid-phase chemiluminescence immunoassay for plasma progesterone.

Author

Kohen F, Kim JB, Lindner HR, and Collins WP

Subjects
Animals, Immunoassay methods, Luminescent Measurements, Phthalazines, Rabbits, Luminol analogs & derivatives, Progesterone blood
Abstract

A solid-phase immunoassay procedure for the determination of progesterone in human plasma is described, which utilizes chemiluminescence as the end-point. A progesterone-isoluminol conjugate serves as the chemiluminescent marker. An IgG fraction of antiserum to progesterone-11 alpha-hemisuccinate bovine serum albumin is passively adsorbed to the walls of Lumacuvettes P polystyrene test tubes. After the binding reaction, the cuvettes are washed. The light yield of the bound conjugate upon oxidation with a H2O2-microperoxidase system at pH 13 decreased with increasing free progesterone concentration in a log-linear manner over the range 15-1000 pg/tube. The chemiluminescence immunoassay is comparable to radioimmunoassay with regard to sensitivity, specificity, precision and accuracy. The assay offers the advantages of speed and ease of automation. In addition, this method does not involve the use of radioisotopes or of a centrifugation step.

Published
1981
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253. Hydrocortisone inhibits antigen-induced rise in intracellular free calcium concentration and abolishes leukotriene C4 production in leukemic basophils.

Author

Zor U, Her E, Talmon J, Kohen F, Harell T, Moshonov S, and Rivnay B

Subjects
Animals, Basophils metabolism, Cell Line, Leukemia, Experimental metabolism, Spectrometry, Fluorescence, Tumor Cells, Cultured metabolism, Antigens immunology, Basophils drug effects, Calcium metabolism, Hydrocortisone pharmacology, SRS-A biosynthesis
Abstract

Antigenic stimulation of rat basophilic leukemia cells (RBL-3H3) elevates intracellular free Ca2+ concentration ([Ca2+]i) and induces production of leukotriene C4 (LTC4). This model was used to examine the role of Ca2+ in LTC4 formation, and inhibition by hydrocortisone (HC). HC, at a physiological concentration (2 x 10(-7) M), selectively prevented the stimulatory effect of the antigen on LTC4 production whereas the response to calcium ionophore (A23187) remained unimpaired. The inhibition by HC was time-dependent: half maximal response was reached at 2 hour and maximal response at 3 hours. Addition of arachidonic acid (3 micrograms/ml) did not overcome the inhibitory action of HC. An elevated [Ca2+]i is known to be essential for the activation of both 5-lipoxygenase and phospholipase A2. The stimulatory effect of the antigen on LTC4 production was abolished when the cells were incubated in Ca2+-deficient medium. Likewise, calcium ionophore stimulation shows dependence on extracellular Ca2+. Half maximal stimulation by the antigen and calcium ionophore was observed at external Ca2+ concentration of 150 microM and 40 microM respectively. Treatment with HC largely prevented the antigen-induced rise in [Ca2+]i, measured by Quin 2. In addition, HC reduced by 70% the accumulation of 45Ca2+ induced by the antigen. Collectively, these results demonstrate for the first time that HC reduces antigen-induced elevation of [Ca2+]i, and this may be associated with the inhibitory action of HC on LTC4 formation. This property could be partly responsible for the antiallergic and antiinflammatory activities of HC.

Published
1987
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254. Immunometric assay for lutropin (hLH) based on the use of universal reagents for enzymatic labelling and magnetic separation and monitored by enhanced chemiluminescence.

Author

Pazzagli M, Kohen F, Sufi S, Masironi B, and Cekan SZ

Subjects
Antibody Specificity, Binding Sites, Antibody, Humans, Indicators and Reagents, Kinetics, Luteinizing Hormone immunology, Luteinizing Hormone standards, Reference Standards, Antibodies, Anti-Idiotypic, Horseradish Peroxidase, Immunoassay methods, Immunoassay standards, Immunoglobulin G immunology, Luminescent Measurements, Luteinizing Hormone analysis, Magnetics, Peroxidases
Abstract

A solid-phase immunometric assay of human lutropin (hLH) is described. Two different anti-hLH antibodies were utilized as capture antibodies, and anti-IgG antibodies covalently coupled to magnetic particles and horseradish peroxidase, respectively, served as 'universal' detection reagents. An anti-hLH antibody raised in rabbits was incubated with a goat anti-rabbit IgG covalently bound to magnetic particles. The resulting complex was added to a separately incubated mixture of hLH and monoclonal anti-hLH antibody. Following incubation, the immunocomplex was sedimented in a magnetic field and the supernatant discarded. Finally a sheep anti-mouse antibody (F(ab')2 fragment) conjugated to horseradish peroxidase as label was added. Following a further incubation, the particles were sedimented in the magnetic field and washed. The hLH content of the sample was quantitated by measuring 'enhanced chemiluminescence'. The sensitivity of the assay was 2.5 +/- 0.9 IU/l (mean +/- SD), the within-run variation ranged from 7.9 to 11%, the between-run variation from 12.9 to 19.8%. Cross-reaction with hFSH or hTSH could not be detected, but was approximately 0.1% with hCG. The results correlated well with those obtained by radioimmunoassay (r = 0.84).

Published
1988
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255. Monitoring ovarian function by a solid-phase chemiluminescence immunoassay.

Author

Weerasekera DA, Kim JB, Barnard GJ, Collins WP, Kohen F, and Lindner HR

Subjects
Adsorption, Antibodies analysis, Calibration, Estrogens, Conjugated (USP) urine, Estrone analogs & derivatives, Estrone urine, Female, Humans, Immunoglobulin G analysis, Luminescent Measurements, Menstruation, Monitoring, Physiologic, Radioimmunoassay, Sodium Hydroxide pharmacology, Immunoassay methods, Ovary physiology
Published
1982
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256. The measurement of urinary LH, by a solid-phase chemiluminescence immunoassay.

Author

Brockelbank JL, Kim JB, Barnard GJ, Collins WP, Gaier B, and Kohen F

Subjects
Buffers, Female, Follicular Phase, Humans, Immunoassay methods, Immunoglobulin G analysis, Luminescent Measurements, Ovulation, Quality Control, Ultrasonography, Luteinizing Hormone urine
Abstract

Ovulation in women may be predicted or detected by a simple, solid-phase, chemiluminescence immunoassay for the measurement of urinary LH. An IgG fraction of a donkey antiserum to rabbit immunoglobulins is passively adsorbed to the walls of polystyrene tubes. Human chorionic gonadotrophin-succinyl-butyl-ethyl-isoluminol and a primary antibody (rabbit anti-human LH) is incubated with samples of early morning urine. After the binding reaction, the solution is removed by aspiration. The antibody-bound fraction is washed twice with buffer. Sodium hydroxide is added and the mixture incubated. After cooling, luminescence is initiated by oxidation of the label with microperoxidase/hydrogen peroxide and the signal integrated. The method has been evaluated in terms of sensitivity, within- and between-batch precision, bias and parallelism. The time interval between the peak day of LH in EMU and maximum follicular diameter during 38 menstrual cycles was -24 h (11%), O h (50%), + 24 h (28%) and + 48 h (11%).

Published
1984
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257. Chemiluminescent labelled streptavidin (STAV) as a universal marker in steroid and peptide immunoassays.

Author

Strasburger CJ and Kohen F

Subjects
Antigens analysis, Biotin, Haptens analysis, Luminol analogs & derivatives, Peptides analysis, Steroids analysis, Streptavidin, Bacterial Proteins, Immunoassay methods, Luminescent Measurements
Abstract

The tetrameric structure of streptavidin and its exceptionally strong affinity to biotin (Ka = 10(15)M 1) can be exploited to achieve an amplification of the signal in immunoassays. In the approach described here streptavidin (STAV) labelled with aminobutylethyl-isoluminol (ABEI) served as a universal marker in immunoassays for both haptens and big antigens. The advantageous features of streptavidin can be applied to any immunoassay using biotinylated antibodies as the primary probe. In two-site immunometric assays for larger antigens the liquid phase 'tracer' antibody is biotinylated. In hapten assays the solid phase antigen technique (Wood et al., 1982) is employed, in which sample-antigen and solid phase-antigen compete for a biotinylated antibody. In this paper we demonstrate the use of STAV-ABEI as a universal chemiluminescent label in steroid assays and in an immunometric assay using human growth hormone (hGH) as an example.

Published
1989
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258. The effect of human monocytes and macrophages on lymphocyte proliferation.

Author

Passwell JH, Levanon M, Davidsohn J, Kohen F, and Ramot B

Subjects
Candida immunology, Cell Division, Cells, Cultured, Dinoprostone, Endotoxins pharmacology, Humans, Leukocyte Count, Lymphocytes immunology, Prostaglandins E analysis, Tuberculin immunology, Zymosan pharmacology, Lymphocyte Activation drug effects, Macrophages immunology, Monocytes immunology
Abstract

Human monocytes suppressed both the phytohaemagglutin (PHA) or antigen-induced lymphocyte proliferative response, when the monocyte: lymphocyte ratio was increased or when the monocytes were stimulated with zymosan or endotoxin. The effect of monocytes on autologous lymphocyte proliferation was compared with that of macrophages obtained by culturing monocytes in vitro for 7 days. The lymphocyte proliferative responses were increased in the presence of macrophages, however, neither increasing their number nor stimulation by zymosan or endotoxin altered the autologous lymphocyte proliferative response to PHA or purified protein derivative (PPD). The PGE2 concentration in the medium of both the cultured monocytes or macrophages activated by zymosan and endotoxin rose markedly without a corresponding suppressor effect on lymphocyte proliferation in the presence of macrophages in the culture. Thus it seems that while PGE2 is a useful marker of mononuclear phagocyte activation, other molecular species are of importance in determining the lymphocyte proliferative response to mitogens and antigens.

Published
1982

259. Gonadotropin-induced differentiation of granulosa cells is associated with the co-ordinated regulation of cytoskeletal proteins involved in cell-contact formation.

Author

Ben-Ze'ev A, Kohen F, and Amsterdam A

Subjects
Animals, Cell Adhesion drug effects, Cell Differentiation drug effects, Cells, Cultured, Cyclic AMP metabolism, Cytochalasins pharmacology, Female, Granulosa Cells cytology, Granulosa Cells metabolism, RNA, Messenger metabolism, Rats, Steroids biosynthesis, Cytoskeletal Proteins metabolism, Gonadotropins pharmacology, Granulosa Cells drug effects
Abstract

The gonadotropin-induced differentiation of granulosa cells in culture was studied, with particular attention being given to the organization and expression of cytoskeletal proteins involved in the formation of cell contacts, as well as to progesterone production. Gonadotropin-treated granulosa cells formed clusters of spherical cells containing few vinculin-containing focal contacts, exhibited a diffuse distribution of actin, and had few adherens junctions but more gap junctions than cells grown without the hormone. In gonadotropin-treated cells, the levels of synthesis of the cytoskeletal proteins, vinculin, alpha-actinin, and actin, were dramatically reduced, but the synthesis of the tubulins and vimentin was unaffected. Decreased levels of synthesis of these cytoskeletal proteins were also observed in an in vitro translation assay using poly(A)+ RNA from gonadotropin-treated cells. The hybridization of cytoplasmic RNA with cloned actin and vimentin cDNAs revealed a marked decrease in actin-RNA levels, but no change in vimentin-RNA levels in these cells. Such alterations in cytoskeletal-protein expression were also observed in cells treated with compounds that cause elevated cellular cAMP levels by acting at a stage beyond gonadotropin receptor stimulation. Furthermore, by keeping the cells in a spherical configuration in suspension culture, or by treating the cells with cytochalasin B, similar changes in the synthesis of these cytoskeletal proteins were observed. During this process, there was a concomitant increased in the production of progesterone (although to a much lesser extent in suspension culture) that occurred in parallel with the appearance of large mitochondria with lamellar-tubular cristae and a well-developed smooth endoplasmic reticulum, these features being characteristic of granulosa-lutein cells in vivo. Our results suggest that changes in cell shape and contact, together with the regulation of cytoskeletal elements that determine cellular morphogenesis, are part of the gonadotropin-controlled differentiation program in granulosa cells and may also occur during the maturation of these cells in vivo.

Published
1987
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260. Antitumor effects of inhibitors of arachidonic acid cascade on experimentally induced intestinal tumors.

Author

Birkenfeld S, Zaltsman YA, Krispin M, Zakut H, Zor U, and Kohen F

Subjects
Animals, Arachidonic Acids antagonists & inhibitors, Intestinal Neoplasms chemically induced, Male, Methylazoxymethanol Acetate analogs & derivatives, Prostaglandin Antagonists, Rats, Rats, Inbred Strains, Catechols therapeutic use, Indomethacin therapeutic use, Intestinal Neoplasms drug therapy, Masoprocol therapeutic use
Abstract

The antitumor action of inhibitors of cyclooxygenase (indomethacin) and lipoxygenase activity (nordihydroguaiaretic acid) of arachidonic acid cascade was investigated in the chemically induced large bowel tumors in Sprague-Dawley rats. Indomethacin treatment completely prevented the carcinogenic effect of methylazoxymethanol. Thus, no tumors were found in the 14 rat test group, compared with 13 of 14 tumor-bearing rats in the untreated control group. Although nordihydroguaiaretic acid treatment does not abolish prostaglandin synthesis, it does reduce the effect of the carcinogen and tumors were found in only five of 14 treated rats. From this study it can be postulated that not only is reduction in prostaglandin formation responsible for the inhibition of tumor growth, but also leukotrienes may play some role.

Published
1987
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261. Antibodies to spiroperidol and their anti-idiotypes as probes for studying dopamine receptors.

Author

Schreiber M, Fogelfeld L, Souroujon MC, Kohen F, and Fuchs S

Subjects
Animals, Antibodies isolation & purification, Antibody Specificity, Cattle, Corpus Striatum immunology, Rabbits immunology, Rats, Serum Albumin, Bovine immunology, Antibodies immunology, Butyrophenones immunology, Immunoglobulin Idiotypes immunology, Receptors, Dopamine immunology, Spiperone immunology
Abstract

Spiroperidol was covalently conjugated to bovine serum albumin (BSA). Conjugated spiroperidol was almost as efficient as free spiroperidol in its binding capacity to dopamine receptor. Antibodies to spiroperidol were produced in rabbits following repeated immunizations with the conjugate of spiroperidol and BSA. The obtained antibodies have an apparent KD of 0.02 nM for [3H]-spiroperidol. These antibodies bind also to other butyrophenones with IC50 values three to four orders of magnitude higher than the IC50 obtained with unlabeled spiroperidol. Antibodies were purified from anti-spiroperidol sera by affinity chromatography. Anti-idiotypic antibodies were raised in rabbits by immunization with the purified anti-spiroperidol antibodies. Some rabbits produced anti-idiotypic antibodies which bind to rat and calf striatum.

Published
1983
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262. Use of monoclonal antibodies to pregnanediol-3 alpha-glucuronide for the development of a solid phase chemiluminescence immunoassay.

Author

Eshhar Z, Kim JB, Barnard G, Collins WP, Gilad S, Lindner HR, and Kohen F

Subjects
Animals, Antibodies, Monoclonal, Chromatography, Gas, Female, Glucuronates immunology, Glucuronates urine, Humans, Hybrid Cells immunology, Immunoassay methods, Immunoglobulin G metabolism, Luminescent Measurements, Male, Menstruation, Mice, Multiple Myeloma metabolism, Neoplasms, Experimental metabolism, Pregnanediol immunology, Pregnanediol urine, Temperature, Time Factors, Pregnanediol analogs & derivatives
Abstract

Monoclonal antibodies to pregnanediol-3 alpha-glucuronide were produced by hybridomas between P3-X63-Ag8 variants and spleen cell of mice immunized with a bovine serum albumin conjugate of the homologous hapten. The ascites fluid collected from mice inoculated with the cloned hybridoma cells contained antibodies with high specificity and affinity to pregnanediol-3 alpha-glucuronide. A sensitive solid-phase chemiluminescence immunoassay for urinary pregnanediol-3 alpha-glucuronide was established utilizing these antibodies. The assay was validated in terms of specificity, accuracy, sensitivity and precision. When urine samples were assayed for pregnanediol-3 alpha-glucuronide, the results obtained by the solid-phase chemiluminescence immunoassay method and the conventional gas liquid chromatographic method agreed well (n = 30, r = 0.96). The method may be of value for monitoring luteal function since it is fast, sensitive and does not require the use of radioisotopes or purification of the biological sample. Monoclonal antibody preparations facilitate rigorous standardization of the assay.

Published
1981
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263. Studies on human milk macrophages: effect of activation on phagocytosis and secretion of prostaglandin E2 and lysozyme.

Author

Blau H, Passwell JH, Levanon M, Davidson J, Kohen F, and Ramot B

Subjects
Concanavalin A pharmacology, Female, Humans, Hydrogen-Ion Concentration, In Vitro Techniques, Macrophages physiology, Macrophages metabolism, Milk, Human cytology, Phagocytosis, Prostaglandins E biosynthesis, Zymosan biosynthesis
Abstract

Breast milk macrophages cultured in vitro synthesized and secreted increasing amounts of protein, lysozyme, and prostaglandin E2(PGE2) into the extracellular medium. These cells were also shown to actively phagocytose labeled zymosan particles in culture. Morphologic characteristics, phagocytosis, and secretory responses of the macrophages were altered depending on the presence of various stimuli in the culture. Concanavalin A, endotoxin and zymosan particles, but not latex particles, all resulted in an increased PGE2 secretion into the medium. Although total protein synthesis was not altered by any of these stimuli, Concanavalin A and endotoxin resulted in a decreased lysozyme concentration in the extracellular medium. Concanavalin A enhanced, whereas endotoxin and prior phagocytosis of latex particles inhibited phagocytosis of labeled zymosan particles. These findings indicate that phagocytosis and secretions of milk macrophages may be altered depending on the nature of the stimulating agent.

Published
1983
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264. Measurement of estrone-3-glucuronide in urine by rapid, homogeneous time-resolved fluoroimmunoassay.

Author

Barnard G, Kohen F, Mikola H, and Lövgren T

Subjects
Antibodies, Monoclonal, Antibody Specificity, Estrone urine, Europium, Female, Fluorescent Dyes, Fluorometry, Humans, Quality Control, Radioimmunoassay, Estrone analogs & derivatives, Immunoassay
Abstract

We describe a liquid-phase nonseparation time-resolved fluorescence immunoassay for measuring estrone-3-glucuronide in undiluted urine. The sensitivity, specificity, and accuracy are similar to those for a conventional separation fluoroimmunoassay or radioimmunoassay, but the speed, convenience, precision, reliability, and clinical utility of the new method are more advantageous. The labeled antigen, a fluorescent europium chelate covalently linked to estrone-3-glucuronide, is incubated for 10 min with a limited concentration of polyclonal or monoclonal antibodies to estrone-3-glucuronyl-6-bovine serum albumin and 10 microL of standard or sample (undiluted urine) in microtiter wells. The fluorescence emanating from the antibody-free label, which is proportional to the concentration of estrone-3-glucuronide in the standard or sample, is then measured in a time-resolved fluorometer. The method is useful for monitoring ovarian function in women.

Published
1989

265. A thiophilic adsorbent for the one-step high-performance liquid chromatography purification of monoclonal antibodies.

Author

Nopper B, Kohen F, and Wilchek M

Subjects
Adsorption, Animals, Electrophoresis, Polyacrylamide Gel, Fluoroimmunoassay, Immunoglobulin G isolation & purification, Male, Mice, Rats, Silicon Dioxide, Sulfhydryl Compounds, Antibodies, Monoclonal isolation & purification, Chromatography, High Pressure Liquid methods
Abstract

Thiophilic adsorption chromatography, developed originally by Porath and colleagues (1985, FEBS Lett. 185, 306-310) for conventional chromatographic techniques, was transformed to the HPLC mode upon preparation of new and improved sulfur-containing silica beads. The new thiophilic adsorbent is of high capacity and is suitable for the rapid and single-step purification of all subclasses of monoclonal and polyclonal antibodies. Due to its broad specificity, the thiophilic silica column is an efficient, stable, and inexpensive substitute for protein A and protein G columns used today to purify antibodies.

Published
1989
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270. Hypocholesterolemic agents. 7. The C-17 epimer of 20,25-diazacholesterol.

Author

Ranade VV, Kohen F, and Counsell RE

Subjects
Androstanes analysis, Androstanes chemical synthesis, Chemical Phenomena, Chemistry, Models, Structural, Stereoisomerism, Anticholesteremic Agents analysis, Anticholesteremic Agents chemical synthesis, Anticholesteremic Agents pharmacology, Cholesterol chemical synthesis, Cholesterol pharmacology
Published
1971
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271. Regulation of human gonadotropins. 8. Suppression of serum LH and FSH in adult males following exogenous testosterone administration.

Author

Lee PA, Jaffe RB, Midgley AR Jr, Kohen F, and Niswinder GD

Subjects
Adult, Animals, Cattle immunology, Depression, Chemical, Humans, Injections, Intramuscular, Iodine Isotopes, Male, Methods, Radioimmunoassay, Sex Factors, Testosterone administration & dosage, Testosterone blood, Tritium, Follicle Stimulating Hormone blood, Luteinizing Hormone blood, Testosterone pharmacology
Published
1972
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