Your search keyword '"Holmes SD"' showing total 7 results

1. Delta-9-tetrahydrocannabinol stimulates ABP secretion from rat Sertoli cells in vitro.

Author

Holmes SD, Lipshultz LI, and Smith RG

Subjects

Animals, Bucladesine pharmacology, Cells, Cultured, Dose-Response Relationship, Drug, Electrophoresis, Polyacrylamide Gel, Follicle Stimulating Hormone pharmacology, Male, Plasminogen Activators analysis, Rats, Rats, Inbred Strains, Sertoli Cells metabolism, Spermatozoa drug effects, Stimulation, Chemical, Testosterone pharmacology, gamma-Glutamyltransferase analysis, Androgen-Binding Protein metabolism, Dronabinol pharmacology, Sertoli Cells drug effects

Abstract

The effect of delta-9-tetrahydrocannabinol (THC) on rat Sertoli cell function was investigated. THC significantly increased ABP secretion by 1.5- to 2.1-fold but did not consistently enhance the stimulation of ABP induced by FSH, testosterone or dibutyryl cyclic AMP. ABP was measured by steady-state polyacrylamide gel electrophoresis, DEAE Bio-Gel and immunoassay; all three methods gave similar results. The minimal concentration of THC that stimulated ABP was 10 ng/ml; maximal stimulation was observed with 100-200 ng/ml. This effect was specific since THC did not affect gamma glutamyl transpeptidase activity or the secretion of plasminogen activator, lactate and transferrin. This observation that THC affects ABP secretion specifically is the first report of any differential effect of a drug on Sertoli cell secretion.

Published

1986

2. Effect of cannabinoids on human Sertoli cell function in vitro.

Author

Holmes SD, Lipshultz LI, and Smith RG

Subjects

Acyltransferases metabolism, Cannabidiol pharmacology, Cannabinol pharmacology, Cells, Cultured, Dose-Response Relationship, Drug, Follicle Stimulating Hormone pharmacology, Humans, In Vitro Techniques, Iron pharmacology, Kinetics, Male, Sertoli Cells physiology, Testosterone pharmacology, Transferrin metabolism, Transglutaminases, Cannabinoids pharmacology, Dronabinol pharmacology, Sertoli Cells drug effects

Abstract

Exposure to marijuana adversely affects spermatogenesis in humans and rodents. Since the Sertoli cell interfaces between changes in the serum hormonal milieu and the adluminal compartment and acts in various ways to support the germinal epithelium, this adverse marijuana mediated effect might be transmitted locally in the testes of humans by interference with Sertoli cell function. This report describes the effect of three active marijuana components: delta-9-tetrahydrocannabinol (THC), cannabidiol (CD) and cannabinol (CN) on various human Sertoli cell markers: transferrin, protein secretion and gamma glutamyl transpeptidase activity utilizing cultured human Sertoli cells. THC, CD, and CN tested in concentrations up to 200 ng/ml did not change transferrin secretion by these human Sertoli cells. Transferrin represents 1-4% of the total newly synthesized proteins of human Sertoli cells in culture. Even when the Sertoli cells were incubated for 30 days with THC there was no effect on transferrin secretion. The presence or absence of follicle-stimulating hormone, testosterone (T) or Fe3+ in the culture media did not modify the effect of THC. THC, CD, and CN also did not alter total protein secretion by Sertoli cells nor affect the level of gamma glutamyl transpeptidase activity.

Published

1983

3. Rat Sertoli cells secrete a growth factor that blocks epidermal growth factor (EGF) binding to its receptor.

Author

Holmes SD, Spotts G, and Smith RG

Subjects

Animals, Cell Division drug effects, Cell Line, Chromatography, Gel, Chromatography, High Pressure Liquid, Dose-Response Relationship, Drug, ErbB Receptors, Growth Substances metabolism, Male, Mice, Molecular Weight, Spermatogenesis, Epidermal Growth Factor metabolism, Growth Substances pharmacology, Receptors, Cell Surface drug effects, Sertoli Cells metabolism

Abstract

The conditioned medium from Sertoli cells contains a potent mitogen(s) that can markedly stimulate the proliferation of 4 different cell lines of endoderm or mesoderm origin in the presence or absence of serum. With A431 cells, conditioned medium produced in a dose-dependent manner up to a 5.2-fold increase in cell number after 5 days in culture. Addition of follicle-stimulating hormone (FSH), testosterone, retinol, and insulin to the Sertoli cells increased the secretion of the mitogenic activity. The ability of Sertoli cell conditioned medium (SCCM) to displace 125I-labeled epidermal growth factor (125I-EGF) from formalin-fixed A431 cells was also examined. The SCCM from Sertoli cells incubated with insulin contained 1.42 ng eq of EGF/ml; testosterone, retinol, and FSH (in the presence of insulin) further increased the secretion of this EGF competing activity to 2.09, 2.56, and 3.22 ng eq/ml, respectively. The amount of EGF competing activity was positively correlated with mitogenic activity. Separation of SCCM by gel filtration on Bio-Gel P-10 produced three major peaks of EGF-competing activity at apparent Mr = 1800-2100, 3800-4200, and 8000-9500. Chromatographing SCCM (in the presence of protease inhibitors) on size exclusion high performance liquid chromatography revealed two peaks of EGF competing activity at Mr about 8000 and 2000 coincident with and proportional to peaks of mitogenic activity. This activity was heat-sensitive and resistant to reducing agents, and addition of an equivalent amount of EGF as that present in SCCM produced an inhibition in growth of the A431 cells compared to a 3-fold stimulation with SCCM. Thus, the Sertoli cells secrete a potent mitogen that is distinct from EGF and alpha TGF. This factor that we have termed Sertoli cell-secreted growth factor is hormonally regulated by FSH, testosterone, and retinol and may play an important role in controlling spermatogenesis.

Published

1986

4. Regulation of transferrin secretion by human Sertoli cells cultured in the presence or absence of human peritubular cells.

Author

Holmes SD, Lipshultz LI, and Smith RG

Subjects

1-Methyl-3-isobutylxanthine pharmacology, Bucladesine pharmacology, Cells, Cultured, Follicle Stimulating Hormone pharmacology, Humans, Insulin pharmacology, Male, Seminiferous Tubules, Testis cytology, Time Factors, Sertoli Cells metabolism, Testis physiology, Transferrin metabolism

Abstract

Transferrin represents 1-4% of the total proteins secreted by human Sertoli cells, and the amount secreted by the cells was maximal after a 4- to 5-day period in culture, the time chosen for each medium change. During this first 4- to 5-day period, the addition of FSH, insulin, (Bu)2cAMP, and isobutylmethylxanthine had no effect on transferrin secretion; however, from days 4-5 to 8-10, each of the above compounds significantly stimulated transferrin secretion compared to control values. Testosterone (in the absence or presence of insulin) had no effect. Transferrin secretion increased for the first 5 days in culture, with a similar magnitude in the presence or absence of the above stimulators, and thereafter declined, more so in untreated cultures. These results suggest that these agents do not stimulate, but, rather, limit the decline in transferrin secretion. When human peritubular cells were cocultured with Sertoli cells, transferrin secretion was significantly elevated compared to that by Sertoli cells alone. Interestingly, in the cocultures (Bu)2cAMP stimulated transferrin secretion when added for the first 4- to 5-day culture period. Human fibroblasts or spent medium from the peritubular cell cultures did not mimic the effect found when peritubular and Sertoli cells were cocultured. These results provide evidence that peritubular cells play a critical role in regulating human Sertoli cell function.

Published

1984

5. Rapid method for quantitation of androgen binding protein in Sertoli cell cultures and its use for measurement of binding kinetics.

Author

Johnson AR, Holmes SD, Lipshultz LI, and Smith RG

Subjects

Adsorption, Androgen-Binding Protein metabolism, Animals, Cells, Cultured, Dihydrotestosterone metabolism, Electrophoresis, Polyacrylamide Gel, Ethanolamines, Filtration, Hydroxyapatites, Kinetics, Male, Methods, Rats, Rats, Inbred Strains, Sertoli Cells metabolism, Androgen-Binding Protein analysis, Carrier Proteins analysis, Sertoli Cells analysis

Abstract

The accurate measurement of the kinetics of binding of 5 alpha-dihydrotestosterone to the Sertoli cell specific protein, androgen binding protein (ABP), has been frustrated by the extremely rapid rate of dissociation of the ABP-dihydrotestosterone complex. We describe a rapid and highly sensitive assay suitable for ABP quantitation which utilizes DEAE Bio-Gel and [3H]dihydrotestosterone. The assay has been used to accurately measure the rate of dissociation (8.25 X 10(-4) s-1, t1/2 14 min) and the rate of association (2.04 X 10(5) M s-1) of the binding of [3H]dihydrotestosterone to rat ABP. The ratio of these rate constants is in perfect agreement with the equilibrium dissociation constant determined by Scatchard analysis (4.0 nM). This multipoint assay is extremely rapid such that binding can be measured at equilibrium, it has high precision (coefficient of variation 3%), and is particularly useful at low protein concentrations (50 ng/ml); furthermore, the assay background of nonspecific 3H-binding is extremely low (0.2%). Since at such low protein concentrations a 10 point Scatchard analysis can be performed on 1 ml culture medium containing as little as 3 fmol ABP, the assay is suitable for monitoring changes in ABP secretion resulting from manipulations of cells in culture. The assay which utilizes DEAE Bio-Gel A is compared to five alternative methods: the standard method of steady state gel electrophoresis, Dextran-coated charcoal assay, hydroxylapatite assay, DEAE filter assay, and radioimmunoassay. The DEAE Bio-Gel assay has advantages over all of these alternative methods. In summary, this new assay is particularly useful for monitoring temporal changes in the secretion of ABP, and the method is equally effective in quantitating ABP in rat, rabbit and hamster Sertoli cell cultures.

Published

1985

6. Characterization of a growth factor secreted by rat Sertoli cells in culture.

Author

Holmes SD, Spotts G, and Smith RG

Subjects

Androgen-Binding Protein metabolism, Animals, Cells, Cultured, Follicle Stimulating Hormone pharmacology, Male, Rats, Sertoli Cells cytology, Sertoli Cells drug effects, Transferrin metabolism, Growth Substances metabolism, Sertoli Cells metabolism

Published

1986

7. Transferrin and gonadal dysfunction in man.

Author

Holmes SD, Lipshultz LI, and Smith RG

Subjects

Follicle Stimulating Hormone blood, Humans, Infertility, Male etiology, Male, Oligospermia metabolism, Testicular Diseases diagnosis, Testicular Diseases metabolism, Infertility, Male metabolism, Semen analysis, Sertoli Cells metabolism, Transferrin analysis

Abstract

Transferrin concentrations were quantitated in the seminal fluid of normal, oligozoospermic, and azoospermic patients and related to other known parameters of testicular function. Transferrin concentration in the semen of patients 2 months after vasectomy (13.2 +/- 1.8 micrograms/ml) was significantly less than that obtained from pregnancy-proven donors (65.6 +/- 10.1 micrograms/ml). This indicates that approximately 80% of the seminal fluid transferrin is derived from the testes. The concentration of transferrin in semen from patients with azoospermia (14.4 +/- 1.8 micrograms/ml), severe oligozoospermia (17.5 +/- 1.7 micrograms/ml), and moderate oligozoospermia (21.8 +/- 4.3 micrograms/ml) was significantly lower than normospermic groups. Serum follicle-stimulating hormone (FSH) was measured in a group of infertile patients; those having an elevated FSH had a significantly lower concentration of semen transferrin, 14.1 +/- 1.6 micrograms/ml, compared with patients who had FSH levels within the normal range (33.7 +/- 5.3 micrograms/ml). It is possible that the underlying cause in decreased spermatogenesis associated with both an elevated FSH and a decreased transferrin concentration is impaired Sertoli cell function.

Published

1982