Your search keyword '"Irving B. Fritz"' showing total 129 results

1. Enzymological determination of free carnitine concentrations in rat tissues

Author

Norman R. Marquis and Irving B. Fritz

Subjects

Biochemistry, QD415-436

Abstract

Purified carnitine acetyltransferase was employed to catalyze the reaction:Carnitine+acetylCoA⇌acetylcarnitine+CoA. In the presence of a known excess of acetyl CoA, free CoA released was determined simultaneously in a coupled spectrophotometric assay. CoA formed was shown to be directly related to carnitine initially present. Rat tissue extracts were analyzed using this method, and μmoles of (–)-carnitine per gram dry weight were found to be 4.87 for heart; 3.14 for brown adipose tissue; 2.68 for skeletal muscle; 1.74 for testes; 1.26 for kidney; 0.55 for brain; and 0.051 for serum. The specificity and accuracy of the determinations are described.

Published

1964

2. Long-chain carnitine acyltransferase and the role of acylcarnitine derivatives in the catalytic increase of fatty acid oxidation induced by carnitine

Author

Irving B. Fritz and Kenneth T.N. Yue

Subjects

Biochemistry, QD415-436

Abstract

Carnitine-H3 or palmitate-C14 incubated with heart muscle preparations was incorporated into a compound that had chromatographic behavior in several systems identical to that of palmitylcarnitine chemically synthesized from palmityl chloride and carnitine. Palmitylcarnitine biosynthesis from palmitic acid and carnitine was dependent upon ATP and CoA in addition to substrates and an enzyme preparation. In contrast, palmityl carnitine formation from palmityl CoA and carnitine did not require ATP or CoA. The following reaction, catalyzed by palmitylcarnitine transferase, was shown to be reversible:Palmitylcarnitine+CoA⇌palmitylCoA+carnitine.General chemical and metabolic properties of palmitylcarnitine were defined. Addition of palmitylcarnitine to heart muscle mitochondria increased respiration more than did addition of palmityl CoA, suggesting that palmitylcarnitine can more readily contribute its acyl group to the fatty acid oxidase system than can exogenous palmityl CoA. Carnitine increased degradation of pa1mityl-l-C14 CoA and steary1-l-C14 CoA to CO2 and increased total oxygen uptake in the absence of ATP if acyl CoA were present. Carnitine did not appreciably enhance respiration or increase conversion of pa1mitate-l-C14 to CO2 in the absence of ATP but did augment palmitate oxidation, as previously reported, when ATP and CoA were added to the system. Results are consonant with the hypothesis that the catalytic stimulation by carnitine of long-chain fatty acid oxidation is mediated via acylcarnitine formation, with subsequent transfer of the acyl group to CoA at the site of the fatty acid oxidase system.

Published

1963

3. Nitric oxide-induced perturbations in a cell culture model of the blood-brain barrier

Author

Roger D. Hurst and Irving B. Fritz

Subjects

Diminution, biology, Physiology, Clinical Biochemistry, Cell Biology, Blood–brain barrier, Nitric oxide, Nitric oxide synthase, Endothelial stem cell, chemistry.chemical_compound, medicine.anatomical_structure, chemistry, Biochemistry, medicine, biology.protein, Biophysics, Transcellular, Intracellular, Methylene blue

Abstract

The actions of an intracellular nitric oxide generator compound on the properties of a co-culture model of the blood-brain barrier are described. Addition of the iron-sulphur cluster nitrosyl Roussin's black salt (RBS, heptanitrosyl-tri-mu3-thioxotetraferrate (1-)) resulted in a rapid and dose-dependent (50-250 microM) decline in the electrical resistance displayed by co-cultures of vascular endothelial cells and C6 glioma cells. The breach in barrier integrity elicited by RBS (250 microM) could be prevented by either haemoglobin (100 microM), methylene blue (200 microM), or by photon-induced inactivation of RBS. In contrast, the nitric oxide synthase inhibitor nitro-L-arginine methyl ester (250 microM) caused no inhibition in the decline in resistance of RBS-exposed cultures. Addition of 8-bromo-guanosine-cyclic monophosphate (500 microM) did not mimic the actions of RBS. Exposure to intense light of co-cultures manifesting a high transcellular electrical resistance resulted in a reduction in tissue resistance which could be prevented by the presence of haemoglobin (100 microM). We conclude that nitric oxide liberated from RBS results in a reversible diminution in the integrity of the endothelial cell barrier in the co-culture system, and we suggest that light-sensitive endogenous nitric oxide generator compounds may be present in intact cells. Possible roles of nitric oxide in blood-brain-barrier function are considered.

Published

1996

4. Properties of an immortalised vascular endothelial/glioma cell co-culture model of the blood-brain barrier

Author

Roger D. Hurst and Irving B. Fritz

Subjects

Osmotic shock, Physiology, Clinical Biochemistry, Cell Biology, Biology, medicine.disease, Microfilament, Blood–brain barrier, Umbilical vein, Cell biology, medicine.anatomical_structure, Glioma, medicine, Tumor necrosis factor alpha, Transcellular, Immortalised cell line

Abstract

In an effort to obtain a useful in vitro model possessing some of the properties of the blood-brain barrier, we have investigated the properties and interactions of immortalized cell lines. Immortalised human umbilical vein endothelial cells (HUVEC-304), in co-culture with rat C6 glioma cells in a two-chambered assembly, form tight junctional complexes, and develop a permeability barrier having a high transcellular electrical resistance. The endothelial cells generate a barrier with greatest integrity in the presence of glioma cells, or in the presence of glioma cell conditioned medium. Under these conditions, the endothelial cells also display pronounced structural changes which do not occur in the absence of glioma cells. Morphological alterations include a flattening of cell shape from a cuboidal-type to a squamous-type of appearance, and a re-organization of F-actin microfilaments. The integrity of the barrier can be reversibly disrupted by osmotic shock or by tumor necrosis factor-alpha (TNF-alpha). We interpret these observations to indicate that co-cultures of immortalized vascular endothelial and C6 glioma cells provide a model for the investigation of cell-cell interactions required for the generation of a barrier having several properties of the blood-brain barrier.

Published

1996

5. Role of laminin in the Morphogenetic cascade during Coculture of sertoli cells with peritubular cells

Author

Pierre S. Tung and Irving B. Fritz

Subjects

Male, endocrine system, Physiology, Cytological Techniques, Clinical Biochemistry, Cycloheximide, chemistry.chemical_compound, Laminin, Testis, Cell Adhesion, medicine, Animals, Rats, Wistar, Close contact, Cell Aggregation, Sertoli Cells, biology, urogenital system, Immune Sera, Cell Biology, Sertoli cell, Fibronectins, Rats, Cell biology, Fibronectin, medicine.anatomical_structure, chemistry, Immunoglobulin G, biology.protein

Abstract

Observations summarized in this article demonstrate an essential role of laminin during the restructuring processes that occur during coculture of Sertoli cells with testicular peritubular cells. The data presented indicate that laminin becomes detectable on the free surfaces of Sertoli cells only after reaggregation of Sertoli cells begins, coincident with the initiation of repolarization at a specific stage of the morphogenetic cascade. We infer that laminin deposited at this time serves as a cohesion molecule that permits peritubular cells to come into close contact with Sertoli cells and subsequently to spread along the free surfaces of Sertoli cells. These conclusions and inferences are based on the following experiments. Cycloheximide-treated peritubular cells in culture in MEM containing cycloheximide readily attach to laminin-coated polystyrene surfaces. By contrast, added peritubular cells do not attach onto monolayers of Sertoli cells in monoculture or onto Sertoli cells plated on top of peritubular cells and maintained in coculture for periods of up to 48 h in cocultures maintained for 6 days, however, labeled peritbular cells readily adhere to the free surfaces of reaggregated Sertoli cells. Laminin, but not fibronectin, appears on the free surfaces of the reaggregated Sertoli cells atthis time, coinciding with the period of initial mound formation. The addition of antilaminin IgG, but not antifibronectin IgG, blocks the attachment of cycloheximide-treated peritubular cells to laminin-coated plates and also blocks the subsequent migration of peritubular cells required to form a monolayer. Similarly, anti-laminin IgG inhibits the attachment and spreading of labeled peritubular cells seeded on the free surfaces of reaggregated Sertoli cells in mounds generated during the morphogenetic cascade. We interpret the combined data to indicate that the appearance of laminin on the free surfaces of Sertoli cells is required to permit peritubular cells to adhere and subsequently to migrate on Sertoli cell surfaces, resulting in the formation of a tubule-like structure. © 1994 Wiley-Liss, Inc.

Published

1994

6. Interactions of sertoli cells with laminin are essential to maintain integrity of the cytoskeleton and barrier functions of cells in culture in the two-chambered assembly

Author

Irving B. Fritz and Pierre S. Tung

Subjects

Male, Physiology, Molecular Sequence Data, Clinical Biochemistry, Cell, In Vitro Techniques, Testicle, Permeability, Receptors, Laminin, Laminin, Cell Adhesion, medicine, Extracellular, Animals, Amino Acid Sequence, Rats, Wistar, Cytoskeleton, Sertoli Cells, biology, Tight junction, Cell Membrane, Cell Polarity, Cell Biology, Sertoli cell, Actins, Rats, Cell biology, medicine.anatomical_structure, Cell culture, Immunologic Techniques, biology.protein, Oligopeptides

Abstract

The addition of anti-laminin IgG to the basal surfaces of rat Sertoli cells in culture in a two-chambered assembly results in a perturbation of F-actin arrangements, including disruption of the pericellular circumferal rings, impairments of the Sertoli cell permeability barrier, and subsequently focal defoliation, followed by cell reaggregation. The pentapeptide YIGSR, which competes with the laminin receptor for laminin (Kleinman and Weeks: Curr. Oph. Cell Biol., 1:964–967, 1989; Graf et al.: Biochemistry, 26:6896–6900, 1987) also elicited focal defoliation of Sertoli cells from the extracellular matrix-coated filter in the two-chambered assembly. Addition of YIGSR to Sertoli cell cultures resulted in cell detachment within 2 to 3 h. In contrast, the irrelevant peptide YIGSE had no detectable effects. The anti-laminin IgG was effective only when added to the chamber in which access was readily available to the basal surfaces of Sertoli cells, but YIGSR was effective when added either to the outer chamber or to the inner chamber. These data were interpreted to indicate that the Sertoli cell barrier generated in the two-chambered assembly allowed a relatively rapid diffusion of YIGSR between chambers, but prevented the rapid equilibration of anti-laminin IgG between compartments. Addition of anti-laminin IgG to the basal, but not to the apical surfaces of Sertoli cells, resulted in more rapid rates of equilibration of [3H]-methoxyinulin and [86Rb]Cl across the Sertoli cell monolayer. This evidence of impairment to the integrity of the barrier was detected prior to the disruption of stress fibers and focal defoliation, but after evidence of dissolution of the circumferal F-actin ring, which occurred within 1 h after addition of anti-laminin IgG. We consider the possibility that a transmembrane link exists between extracellular laminin and cytoskeletal elements which modulates the circumferal F-actin ring. We further postulate that this linkage can influence the nature of tight junctional complexes, and thereby the integrity of the Sertoli cell barrier. © 1993 Wiley-Liss, Inc.

Published

1993

7. Proteases are implicated in the changes in the Sertoli cell cytoskeleton elicited by follicle-stimulating hormone or by dibutyryl cyclic AMP

Author

Pierre S. Tung, Krystyna Burdzy, and Irving B. Fritz

Subjects

Male, endocrine system, medicine.medical_specialty, Proteases, Physiology, Clinical Biochemistry, Biology, Microfilament, Extracellular matrix, Follicle-stimulating hormone, Cell Movement, Internal medicine, Endopeptidases, Testis, medicine, Animals, alpha-Macroglobulins, Cytoskeleton, Actin, Sertoli Cells, Cell Biology, Sertoli cell, Actins, Cell biology, Drug Combinations, Endocrinology, medicine.anatomical_structure, Bucladesine, Cytoplasm, Cattle, Proteoglycans, Collagen, Laminin, Follicle Stimulating Hormone

Abstract

Follicle-stimulating hormone (FSH) or dibutyryl cyclic AMP (dbcAMP) elicits striking morphological changes in Sertoli cells in culture in serum-free medium, resulting in a transition from an epithelial type of cell association pattern to that of an astrocytic or fibroblast-like cell, with attenuated cytoplasmic extensions between cells, and with diminished F-actin stained stress fibers. These responses of Sertoli cells do not occur in the presence of normal untreated serum, but they do take place in the presence of acid-treated serum which is depleted of antiproteases. The addition of alpha 2-macroglobulin to serum-free medium or to antiprotease-depleted serum resulted in the blockage of morphological responses of Sertoli cells to FSH or to dbcAMP. Changes in pattern of arrangements of F-actin in Sertoli cells in culture, which occur in response to FSH or to dbcAMP, were also prevented by the presence of alpha 2-macroglobulin. Thus, the diminution in bundles of F-actin containing stress fibers, which otherwise takes place in Sertoli cells stimulated by FSH or by dbcAMP, did not occur in cells in culture in the presence of alpha 2-macroglobulin, in the presence or absence of acid-treated serum. The inhibiting effects of dbcAMP on the migration of Sertoli cells in serum-free medium became nondetectable in medium containing normal untreated serum, but remained evident in Sertoli cells in culture in medium containing acid-treated serum depleted of antiproteases. Addition of alpha 2-macroglobulin blocked the inhibitory effects of dbcAMP on Sertoli cell migration. Similarly, the presence of alpha 2-macroglobulin prevented the inhibitory effects of dbcAMP on the contractility of TM4 cells which had been embedded in collagen type-I and incubated in serum-free medium. We discuss the possibility that cellular proteases may be implicated in the disintegration of microfilament bundles, either by favoring depolymerization of actin filaments; by facilitating breakage of the link of the transmembrane molecular assembly between cytoskeletal extracellular matrix components; or by catalyzing a disruption of the modular organization of one or more of the actin cross-linking proteins. By inference, we postulate that morphological responses of Sertoli cells to FSH require the activation of cellular proteases for one or more of these reactions, and that alpha 2-macroglobulin blocks the Sertoli cell morphological responses to FSH by inhibiting the proteases involved.

Published

1993

8. Clusterin

Author

Brendan F. Murphy and Irving B. Fritz

Subjects

Endocrinology, Text mining, Clusterin, biology, business.industry, Chemistry, Endocrinology, Diabetes and Metabolism, biology.protein, Computational biology, business

Published

1993

9. High-Resolution scanning electron micrographs of freeze-cracked cells in testes from normal and irradiated rats at different stages of gonadal development

Author

Pierre S. Tung, Irving B. Fritz, and Krystyna Burdzy

Subjects

Male, endocrine system, Pathology, medicine.medical_specialty, Biology, Pregnancy, Testis, medicine, Animals, Freeze Fracturing, Involution (medicine), Sertoli Cells, Rats, Inbred Strains, Seminiferous Tubules, Freeze Etching, Sertoli cell, Spermatozoa, Rats, Cell biology, medicine.anatomical_structure, Cytoplasm, In utero, Microscopy, Electron, Scanning, Ultrastructure, Female, Anatomy, Development of the gonads, Lumen (unit)

Abstract

Newly developed techniques in high-resolution scanning electron microscopy (SEM) and for tissue-processing procedures have been applied to an investigation of structures of various cells in rat testes at different stages of gonadal maturation. A series of high-resolution SEM micrographs are presented which survey the surfaces of different types of testis cells during normal development, and which also illustrate ultrastructural features of some of their intracellular organelles. In addition, a series of high-resolution SEM micrographs are presented which compare the structural features of Sertoli cells in normal testes with those in germ-cell-depleted testes obtained from rats killed at varying times after having been irradiated in utero. We describe our observations on the structural properties of surfaces and intracellular organelles in Sertoli cells, Leydig cells, peritubular myoid cells, and some classes of germinal cells. We also consider the possible role of Sertoli cell apical cytoplasmic processes in lumen formation. Similarities are pointed out between the structure of germ-cell-depleted testes, resulting from irradiation in utero, and the structure of germ-cell-depleted testes in seasonal breeders during periods of involution. Finally, we discuss advantages and disadvantages of methods employed to reveal the fine structure of intracellular organelles in cells of the testis.

Published

1991

10. Transforming growth factor-? and platelet-derived growth factor synergistically stimulate contraction by testicular peritubular cells in culture in serum-free medium

Author

Irving B. Fritz and Pierre S. Tung

Subjects

Male, medicine.medical_specialty, Platelet-derived growth factor, Physiology, medicine.medical_treatment, Clinical Biochemistry, Serum albumin, Contractility, chemistry.chemical_compound, Cell Movement, Transforming Growth Factor beta, Epidermal growth factor, Internal medicine, Testis, medicine, Animals, Bovine serum albumin, Cells, Cultured, Platelet-Derived Growth Factor, biology, Growth factor, Drug Synergism, Cell Biology, Culture Media, Fibronectins, Rats, Endocrinology, chemistry, embryonic structures, biology.protein, Collagen, Platelet-derived growth factor receptor, Transforming growth factor

Abstract

We report investigations on factors influencing contractility by testicular peritubular cells (PC) maintained in culture in a three-dimensional collagen gel system, and the behavior of PC in culture on a two-dimensional system. At low and moderate cell densities, PC embedded in collagen gels in serum-free Eagle's minimal essential medium (MEM) have a lesser degree of contractility than PC in culture in MEM containing calf serum. The contractility by PC, measured by determining changes in diameter of the collagen gel, was increased by addition of transforming growth factor-beta (TGF-beta) to serum-free MEM, and this was further enhanced by supplementing the medium with platelet-derived growth factor (PDGF). In the absence of TGF-beta, however, PDGF had no detectable effects on PC contractility. Other growth factors examined (epidermal growth factor, insulin, and fibroblast growth factor) did not influence the degree of contractility of PC in serum-free MEM in the presence or absence of TGF-beta. PC maintained in MEM supplemented with platelet-poor serum (PPS) have a lesser degree of contractility than their counterparts in MEM containing 2.5% calf serum. The addition of TGF-beta and PDGF to PPS-supplemented MEM restored contractility by PC to a level comparable to that observed by PC in MEM containing complete serum. The addition of nonpurified bovine serum albumin (BSA) to MEM greatly increased PC contractility. By contrast, highly purified BSA had no such effect, suggesting that one or more components adsorbed to the impure BSA was implicated. Polyclonal antibody against fibronectin did not influence the contractility of PC in collagen gels in the presence or absence of serum. Antiserum against TGF-beta partially blocked the enhancement of contractility of PC in MEM containing non-purified BSA. In PC plated on top of a collagen gel lattice, the attachment, spreading, and cell shape were greatly influenced by the presence of TGF-beta and PDGF, both singly and together. Data presented are interpreted to indicate that effects elicited by serum on the properties of PC in culture, and on the contractility of PC, can be attributed in part to the combined influences of TGF-beta and PDGF in serum.

Published

1991

11. Transforming Growth Factor-β Elicits Shape Changes and Increases Contractility of Testicular Peritubular Cells1

Author

Menachem Ailenberg, Irving B. Fritz, and Pierre S. Tung

Subjects

medicine.medical_specialty, Cell Biology, General Medicine, Transforming growth factor beta, Biology, Microfilament, Sertoli cell, Adenosine, Cell biology, Contractility, Paracrine signalling, Endocrinology, Seminiferous tubule, medicine.anatomical_structure, Reproductive Medicine, Internal medicine, medicine, biology.protein, Cytoskeleton, medicine.drug

Abstract

Testicular peritubular cells (PC) in culture in serum-rich Eagle's minimal essential medium (MEM) on a polystyrene substratum proliferate and form fibroblast-like monolayers. The cells assume a flattened shape, and F-actin microfilaments are assembled to form prominent stress fibers. When PC grown under these conditions are dispersed and replated at a low density, a subsequent shift from serum-rich MEM to serum-free MEM results in dramatic changes. Within an hour, the cells round up, the F-actin microfilament assemblies, together with the cytoskeleton, become disrupted, and the degree of contractility is diminished. Under these conditions, addition of transforming growth factor-beta (TGF-beta) results in a more rapid recovery than that observed in cells maintained in basal MEM alone. The presence of TGF-beta results in an increased percentage of cells with flattened shapes during periods between 1 and 6 h after the shift to serum-free MEM. Concomitantly, PC treated with TGF-beta form and maintain well-organized, prominent stress fibers composed of F-actin microfilament bundles. In addition, the degree of contractility of PC embedded in collagen gels and cultured in serum-free MEM is markedly enhanced in cells stimulated by TGF-beta. Treatment of cells with dibutyryl cyclic adenosine 3',5'-monophosphate (dbcAMP) or catecholeamines results in a rounding up of PC in culture, associated with a disruption of microfilament assemblies. Addition of TGF-beta prevents these effects of dbcAMP and beta-agonists, and permits PC to contract. We discuss the physiological significance of observations presented, consider possible mechanisms of action of TGF-beta on PC, and put forward the hypothesis that TGF-beta is one of the paracrine factors in the seminiferous tubule that influence interactions between Sertoli cells and peritubular myoid cells.

Published

1990

12. Somatic Cell-Germ Cell Relationships in Mammalian Testes During Development and Spermatogenesis

Author

Irving B. Fritz

Subjects

endocrine system, urogenital system, Somatic cell, Cell, Biology, Sertoli cell, Cell biology, Paracrine signalling, medicine.anatomical_structure, Meiosis, medicine, Stem cell, Spermatogenesis, Germ cell

Abstract

In the mammalian testis, somatic cells under hormonal regulation greatly influence the different stages of spermatogenesis, both in intermittent breeders and in animals which produce sperm continuously. In turn, specific populations of germinal cells modulate the function of Sertoli cells, the chief somatic cells within mammalian seminiferous tubules. Tubule formation can take place in the absence of germinal cells. Unlike homologous granulosa cells in the ovary, Sertoli cells retain many of their usual functions in germ cell-free animals. Some of the properties of Sertoli cells and their responses to stimulation by androgens or follicle-stimulating hormone are dependent upon information transmitted from neighbouring germinal cells at specific stages of the cycle of the seminiferous epithelium. We review the roles of some of the growth factors and paracrine agents synthesized and secreted by different classes of testicular cells. The potential roles of some of the known factors secreted by Sertoli cells (e.g. activin, inhibin, anti-Mullerian hormones, TGF-beta and somatomedin C) are considered in relation to the control of tubule formation, spermatogonial proliferation and cytodifferentiation, meiosis and the subsequent stages of spermatogenesis. We stress the importance of the unique tubule cytoarchitecture within which cell interactions take place and the changing nature of this cytoarchitecture at different stages of gonadal maturation.

Published

2007

13. Influences of silicates and carnitine-silicate mixtures on the inhibition of aggregation of erythrocytes elicited by the presence of fibrinogen

Author

Pamela V. Ramsohoye and Irving B. Fritz

Subjects

Erythrocytes, Physiology, Clinical Biochemistry, In Vitro Techniques, Medicinal chemistry, Choline, chemistry.chemical_compound, Carnitine, medicine, Humans, Cell Aggregation, Hemagglutination, Silicates, Temperature, Fibrinogen, Cell Biology, Cell aggregation, Silicate, Membrane, Monomer, Hemagglutinins, chemistry, Biochemistry, Polymerization, Sodium hydroxide, medicine.drug

Abstract

Carnitine and acylcarnitine derivatives have been reported to inhibit cell aggregation (Fritz and Burdzy, 1989, J. Cell. Physiol., 140:18-28). A follow-up of these observations showed that whereas the previously described effects of long-chain acylcarnitines were well replicated, those of carnitine on erythrocytes showed marked variability. The latter phenomenon was traced to the presence of silicates in carnitine solutions derived from the use of sodium hydroxide solutions stored in glass containers for the neutralization of carnitine. The present experiments have led to the discovery that oligomeric forms of silicates are powerful inhibitors of red blood cell aggregation which otherwise occurs in the presence of fibrinogen alone. The active form(s) of silicates in this assay, which appear to be generated by polymerization of silicates in metasilicate solutions on neutralization, are unstable and therefore transient under usual conditions. We estimate that the active oligomeric forms contain between 4 to 18 silicon atoms per molecule. When maintained at -18 degrees C in the presence of carnitine, but not in its absence, the active forms of oligomeric silicates remained stable for months, judging from their ability to inhibit cell aggregation. We conclude that carnitine stabilized the oligomeric form(s) of silicate, or that the species stabilized is an oligomeric silicate-carnitine complex. Comparable concentrations of choline, deoxycarnitine, or gamma-aminobutyrate were less effective in stabilizing the active silicate oligomers. The active forms of the silicate oligomers had Ki values of about 10 microM, calculated as the monomeric form, in inhibiting red blood cell aggregation. The data indicate that free carnitine does not directly inhibit erythrocyte inhibition, as previously interpreted, whereas long-chain acylcarnitine derivatives are active in the absence of silicates. Possible mechanism of actions of silicate oligomers on membranes are discussed.

Published

1995

14. Sites of action of carnitine and its derivatives on the cardiovascular system: interactions with membranes

Author

E. Arrigoni-Martelli and Irving B. Fritz

Subjects

Pharmacology, medicine.medical_specialty, Membranes, Fatty acid metabolism, Chemistry, Cardiac muscle, Metabolism, Smooth muscle contraction, Toxicology, medicine.disease_cause, Cardiovascular System, chemistry.chemical_compound, medicine.anatomical_structure, Endocrinology, Internal medicine, Carnitine, medicine, Membrane fluidity, Animals, Humans, Oxidative stress, Ion channel, medicine.drug

Abstract

Carnitine plays an essential role in the regulation of long-chain fatty acid metabolism in skeletal and cardiac muscle, a process that is mediated by well-characterized enzymatic mechanisms. Here, Irving Fritz and Edoardo Arrigoni-Martelli review the evidence that carnitine and its O-acyl derivatives also influence membrane fluidity, ion channel functions, smooth muscle contractility, membrane stability and cardiac functions. The authors present the view that direct interactions of carnitine derivatives with cell membranes are independent of reactions catalysed by carnitine acyltransferases. They propose that the novel actions discussed are implicated in the mechanisms by which carnitine and its derivatives protect perfused hearts subjected to ischaemia or to oxidative stress, and help people suffering from certain types of myocardial ischaemia or peripheral arterial disease.

Published

1993

15. Competition between cell-substratum interactions and cell-cell interactions

Author

Irving B. Fritz, Krystyna Burdzy, Pierre S. Tung, and Katherine Wong

Subjects

Male, Physiology, Clinical Biochemistry, Cell, Cytological Techniques, Peptide, Cell Communication, Biology, Immunofluorescence, Cell Line, Cell–cell interaction, Laminin, Testis, medicine, Animals, Cell Aggregation, Glycoproteins, chemistry.chemical_classification, medicine.diagnostic_test, Clusterin, Sepharose, Cell Biology, eye diseases, Cell biology, Culture Media, medicine.anatomical_structure, chemistry, Cell culture, Immunology, biology.protein, sense organs, Glycoprotein, Oligopeptides, Molecular Chaperones

Abstract

Clusterin, a glycoprotein which elicits the aggregation of a wide variety of cells (Fritz, I.B., and Burdy, K.: J. Cell Physiol., 140:18–28, 1989), has been utilized to investigate some of the factors modulating the competition between cell-substratum interactions and cell-cell interactions. We compared the responses to clusterin by anchorage-independent cells (erythrocytes) with those by anchoragedependent TM4 cells (a cell line derived from neonatal mouse testis cells). Cells were maintained in culture in the presence of various substrata chosen to enhance cell-substratum interactions (laminin-coated wells), or to diminish cell-substratum interactions (agarose-coated wells). Results obtained showed that the aggregation of erythrocytes elicited by clusterin was independent of the nature of the substratum. In contrast, clusterin addition resulted in aggregation of anchorage-dependent TM4 cells only when TM4 cell-substratum interactions were weak. Thus, clusterin did not aggregate TM4 cells plated upon a laminin substratum, but readily aggregated TM4 cells plated upon an agarose-coated substratum, independent of the sequence of addition of cells and clusterin to the culture dish. We utilized YIGSR, a peptide which competes with laminin for laminin receptors, to determine the possible role of laminin receptors on TM4 cells in the competition between cell-substratum interactions and cell-cell interactions. The presence of YIGSR did not alter responses of erythrocytes to clusterin under all conditions examined. In contrast, the responses of TM4 cells to clusterin were greatly changed. YIGSR addition resulted in the inhibition of aggregation of TM4 cells otherwise elicited by clusterin. YIGSR also prevented attachment of TM4 cells to a laminin-coated surface, but this was reversed by the presence of clusterin. We discuss the possible roles of clusterin and laminin in altering the balance in the competition between cell to cell interactions and cell to substratum interactions. © 1992 Wiley-Liss, Inc.

Published

1992

16. Inhibition of cell-cell adhesion and morphogenesis of Dictyostelium by carnitine

Author

Pretty Brar, Irving B. Fritz, and Chi‐Hung Siu

Subjects

Physiology, Clinical Biochemistry, Cell, Morphogenesis, Cell Communication, Dictyostelium discoideum, Choline, Cell–cell interaction, Carnitine, medicine, Cell Adhesion, Animals, Dictyostelium, Cell adhesion, Edetic Acid, Carnitine O-Acetyltransferase, Membrane Glycoproteins, biology, Cell Biology, biology.organism_classification, Cell aggregation, Betaine, medicine.anatomical_structure, Biochemistry, medicine.drug

Abstract

Carnitine (γ-trimethylammonium β-hydroxy-butyric acid) possesses the novel property of preventing cell aggregation elicited by clusterin or by fibrinogen (I.B. Fritz and K. Burdzy, J. Cell. Physiol., 140:18–28 [1989]). In investigations reported here, we show that carnitine also affects cell-cell adhesion in Dicytostelium discoideum, a cellular slime mold whose cells interact in specific and complex manners during discrete stages of development. Two types of cell adhesion systems sequentially appear on the surface of developing Dictyostelium cells, involving the surface glycoprotein gp24 which mediates EDTA-sensitive binding sites, and the surface glycoprotein gp80 which mediates the EDTA-resistant binding sites. Addition of increasing concentrations of D(+)-carnitine and L(-)-carnitine resulted in a progressive inhibition of both the EDTA-sensitive binding sites and the EDTA-resistant binding sites of Dictyostelium cells at different stages of development. In contrast, comparable or higher concentrations of choline, acetyl-β-methylcholine, or deoxycarnitine had no detectable effects on cell aggregation. Concentrations of carnitine required for 50% inhibition of EDTA-resistant adhesion sites were found to be dependent upon levels of gp80 expressed by Dictyostelium, with greatest inhibition by carnitine of reassociation of cells containing the lowest levels of gp80. Removal of carnitine from cells by washing resulted in the rapid restoration of the ability of Dictyostelium to form aggregates and to resume normal development. We discuss possible mechanisms by which carnitine inhibits the aggregation of cells. © 1992 Wiley-Liss, Inc.

Published

1992

17. Clustering of erythrocytes by fibrinogen is inhibited by carnitine: evidence that sulfhydryl groups on red blood cell membranes are involved in carnitine actions

Author

Katherine Wong, Irving B. Fritz, and Krystyna Burdzy

Subjects

Erythrocyte Aggregation, Erythrocytes, Physiology, Clinical Biochemistry, Biology, Fibrinogen, chemistry.chemical_compound, Cell–cell interaction, Carnitine, medicine, Choline, Humans, Sulfhydryl Compounds, Incubation, Glycoproteins, Erythrocyte Membrane, Cell Biology, Red blood cell, Membrane, medicine.anatomical_structure, Clusterin, chemistry, Biochemistry, Human erythrocytes, medicine.drug, Molecular Chaperones

Abstract

Carnitine is bound by intact red blood cells, by red blood cell ghosts, and by glutaraldehyde-fixed human erythrocytes in a non-saturable, temperature-dependent manner. Binding of carnitine by these preparations is blocked by sulfhydryl reagents. Incubation or preincubation of red blood cell preparations with carnitine inhibits the aggregation of erythrocytes otherwise elicited by fibrinogen. Identical effects are obtained with red blood cell ghosts. In contrast, choline, even at high concentrations, is inactive in preventing the aggregation of erythrocytes. We discuss possible mechanisms by which carnitine favors the dispersion of red blood cells, and we present data indicating that sulfhydryl groups on erythrocyte membranes are required to permit these carnitine actions to be manifested.

Published

1991

18. Sertoli cells in culture secrete paracrine factor(s) that inhibit peritubular myoid cell proliferation: identification of heparinoids as likely candidates

Author

Irving B. Fritz and Pierre S. Tung

Subjects

Male, Physiology, Keratan sulfate, Clinical Biochemistry, Mitosis, Biology, Tritium, Cell Line, chemistry.chemical_compound, Paracrine signalling, Mice, Testis, medicine, Animals, Chondroitin sulfate, Glycosaminoglycans, Heparinase, Sertoli Cells, Heparin, Rats, Inbred Strains, Cell Biology, Heparan sulfate, DNA, Glioma, Seminiferous Tubules, Sertoli cell, Growth Inhibitors, Cell biology, Rats, medicine.anatomical_structure, chemistry, Biochemistry, Heparinoids, Cell culture, Heparitin Sulfate, Cell Division, medicine.drug, Thymidine

Abstract

Conditioned medium from Sertoli cells, prepared from testes of 20-day-old rats, contains component(s) that inhibit the incorporation of [3H]-thymidine into DNA of peritubular myoid cells (PMC) and inhibit the proliferation of PMC. These components are trypsin-resistant, heat-stable compounds having a molecular weight less than 30,000. The active inhibitory components in Sertoli cell conditioned medium are inactivated by treatment with heparinase, but not by treatment with hyaluronidase or chondroitin sulfate lyases. Addition of heparin or heparan sulfate results in inhibition of DNA synthesis by PMC in a dose-dependent manner, whereas other glycosaminoglycans (GAGs) examined (hyaluronic acid, keratan sulfate, and chondroitin sulfate) have no detectable effects. Heparin and heparan sulfate are unique among GAGs tested in inhibiting the characteristic multilayer growth pattern of PMC following the attainment of confluence in serum-rich medium. On the basis of these and other data presented, it is concluded that heparin and other heparin-like GAGs synthesized by Sertoli cells are implicated in the modulation of growth of PMC in vitro during co-culture. It is postulated that heparin may play a similar role in maintaining the quiescent peritubular myoid cell phenotype in vivo.

Published

1991

19. Androgens inhibit plasminogen activator activity secreted by Sertoli cells in culture in a two-chambered assembly

Author

Irving B. Fritz, Menachem Ailenberg, and Donna McCabe

Subjects

Male, medicine.medical_specialty, medicine.drug_class, Cytological Techniques, Testicle, Plasminogen Activators, Endocrinology, Internal medicine, medicine, Animals, Insulin, Testosterone, Vitamin A, Cells, Cultured, Sertoli Cells, Chemistry, Androgen, Sertoli cell, Chemically defined medium, medicine.anatomical_structure, Bucladesine, Cell culture, Dihydrotestosterone, Androgens, Steroids, Plasminogen activator, medicine.drug

Abstract

The addition of androgens (testosterone or dihydrotestosterone) resulted in decreased levels of detectable plasminogen activator activity in the medium when Sertoli cells were maintained in culture in a serum-free chemically defined medium in a two-chambered assembly. This occurred in the presence or absence of extracellular matrix or peritubular cells in the system. In the complete two-chambered assembly, addition of androgens simultaneously resulted in a small but significant increase in the integrity of the Sertoli cell barrier separating the two chambers, as indicated by slower rates of equilibration of [3H]methoxyinulin between inner and outer chambers. These responses to steroids appeared to be androgen specific, since other steroids examined (17 beta-estradiol, progesterone, and dexamethasone) had no detectable effects on levels of plasminogen activator activities or on barrier function. We confirmed that when FSH or (Bu)2cAMP is added to stimulate plasminogen activator secretion by Sertoli cells, the integrity of the barrier is decreased, provided no antiproteases are present in the serum-free medium. Simultaneous addition of androgens inhibited these effects of (Bu)2cAMP on Sertoli cells, but did not influence the responses of Sertoli cells to FSH. We compare actions of androgens on Sertoli cells in culture under various conditions and discuss the possible physiological significance of the inhibition of plasminogen activator activity.

Published

1990

20. Inhibition of erythrocyte aggregation by the silicates is reversed by masking the erythrocyte sulphydryl groups

Author

Pamela V. Ramsohoye and Irving B. Fritz

Subjects

Masking (art), Erythrocytes, Chemistry, Silicates, Sulfhydryl Reagents, In Vitro Techniques, Biochemistry, Erythrocyte aggregation, Kinetics, Ethylmaleimide, Biophysics, Humans, Sulfhydryl Compounds, 4-Chloromercuribenzenesulfonate, Cell Aggregation

Published

1997

21. Observations on the binding of androgens by rat testis seminiferous tubules and testis extracts

Author

Irving B. Fritz, Richard G. Vernon, and Bozena Kopec

Subjects

medicine.medical_specialty, genetic structures, Androgen binding, Tubular fluid, Efferent ducts, Biology, Sertoli cell, Biochemistry, Follicle-stimulating hormone, Endocrinology, medicine.anatomical_structure, Internal medicine, Dihydrotestosterone, medicine, biology.protein, Luteinizing hormone, Molecular Biology, Androgen-binding protein, medicine.drug

Abstract

Isolated seminiferous tubules from recently hypophysectomized adult rats rapidly bound 3H-testosterone (T). Analysis of Scatchard plots of the data indicated the existence of at least two androgen binding proteins (ABP), one of which had a high affinity for T and dihydrotestosterone (DHT). The binding capacity of the high affinity ABP was greatly decreased in tubules from regressed hypophysectomized rats, whereas that of the low affinity ABP was increased. Extracts were prepared from homogenates of seminiferous tubules or from whole testes of normal, cryptorchid and hypophysectomized rats, and endogenous androgens were removed from the high speed supernatant fractions by adsorption onto dextran-coated charcoal. Assays for the high affinity ABP (Kd of approximately 10−9 M) indicated relatively high binding capacity in testis extracts from normal or cryptorchid testes, but very low capacities in testis extracts from regressed hypophysectomized rats. In vivo treatment of hypophysectomized animals with follicle stimulating hormone (FSH) increased ABP capacities in testis extracts within 24 h after hormone administration, whereas treatment with luteinizing hormone was less effective. The ABP was shown to be specific for T and DHT. After ligation of the efferent ducts from the testis, ABP of high binding capacity was observed in extracellular extracts. The data are discussed in relation to the hypothesis that Sertoli cells produce ABP and secrete this protein into tubular fluid under the regulation of FSH. A large portion of the high affinity ABP found in testicular extracts is derived from that present in tubular fluid. The remainder is from the cells of the seminiferous tubules, and little or none is in interstitial cell preparations.

Published

1974

22. Follicle-Stimulating Hormone and Testosterone Independently Increase the Production of Androgen- Binding Protein by Sertoli Cells in Culture*

Author

B G Louis and Irving B. Fritz

Subjects

Male, endocrine system, medicine.medical_specialty, medicine.drug_class, Stimulation, Antiandrogen, Andrology, Follicle-stimulating hormone, chemistry.chemical_compound, Endocrinology, Sex Hormone-Binding Globulin, Internal medicine, medicine, Animals, Testosterone, Cyproterone, Cells, Cultured, Androgen-binding protein, Sertoli Cells, Dose-Response Relationship, Drug, biology, Cyproterone acetate, DNA, Sertoli cell, Rats, Androgen receptor, medicine.anatomical_structure, chemistry, biology.protein, Follicle Stimulating Hormone, hormones, hormone substitutes, and hormone antagonists

Abstract

Dose-response curves were obtained for the production of androgen-binding protein (ABP) by Sertoli cells prepared from testes of 20-day-old rats and treated in culture with either FSH or testosterone (T). FSH stimulated ABP production by up to 3.5 times control levels. For NIH-FSH-S11, the ED50 was 3 ng/ml, and for highly purified ovine FSH, the ED50 was 0.066 ng/ml. Addition of T produced a stimulation of up to 3 times control levels; half-maximal response was obtained at a dose of 4 nM. The presence of small numbers of contaminating Leydig cells in some preparations resulted in production of endogenous T, especially when high doses of NIH-FSH, which contains some LH, were employed. A modified preparation method involving exposure of the cells to distilled water reduced the endogenous T production to low levels. In cultures of cells prepared in this way, addition of the antiandrogen cyproterone acetate at a concentration high enough to reduce fractional occupancy of androgen receptors by endogenous T to 0.014 or less had no effect on the stimulation by FSH of ABP production in the cultures. In contrast, cyproterone acetate inhibited stimulation by T of ABP production. We conclude that FSH and T act independently on Sertoli cells from immature rats to increase the secretion of ABP.

Published

1979

23. Myoinositol biosynthesis by Sertoli cells, and levels of myoinositol biosynthetic enzymes in testis and epididymis

Author

Ranga Robinson and Irving B. Fritz

Subjects

Male, Phosphoric monoester hydrolases, Inositol Phosphates, Phosphatase, Biology, Cyclase, chemistry.chemical_compound, Testis, medicine, Animals, Inositol, Cells, Cultured, Epididymis, Sertoli Cells, General Medicine, Metabolism, Sertoli cell, Phosphoric Monoester Hydrolases, Stimulation, Chemical, Rats, Chemically defined medium, medicine.anatomical_structure, Bucladesine, chemistry, Biochemistry, Myo-Inositol-1-Phosphate Synthase

Abstract

Levels of glucose-6-phosphate cyclase (myoinositol-1-phosphate synthase, EC 5.5.1.4) and myoinositol-1-phosphate phosphatase (myoinositol-1-phosphatase, EC 3.1.3.25) were determined in extracts of testes from 10-, 20-, and 30-day-old rats, and in extracts of Sertoli cells, germinal cells, and epididymides. The specific activity of the cyclase was approximately [Formula: see text] that of the phosphatase in all extracts found to contain either enzyme. Among cells in the testis examined, Sertoli cells had highest levels of enzymes required for inositol biosynthesis from glucose, while spermatocytes and round spermatids did not have detectable activity. Spermatozoa from the epididymis also had no detectable cyclase or phosphatase activity. In contrast, extracts of washed epididymides contained exceedingly high specific activities of these enzymes. Primary cultures of Sertoli cells, maintained in a chemically defined medium without added inositol, released inositol into the medium during three successive 24-h periods. The amounts released were greater in cells stimulated by dibutyryl cyclic AMP. Results were interpreted to indicate that inositol in the fluid of seminiferous tubules most probably originates from Sertoli cells, which synthesize inositol from glucose. Additional inositol in the fluid of epididymal tubules could readily be provided by metabolism of glucose by epididymal epithelial cells.

Published

1979

24. Purification and characterization of a cell-aggregating factor (clusterin), the major glycoprotein in ram rete testis fluid

Author

K Burdzy, Orest W. Blaschuk, and Irving B. Fritz

Subjects

biology, Clusterin, Molecular mass, Cell Biology, Sertoli cell, Biochemistry, Molecular biology, eye diseases, Wheat germ agglutinin, Sepharose, medicine.anatomical_structure, Isoelectric point, Affinity chromatography, Concanavalin A, biology.protein, medicine, sense organs, Molecular Biology

Abstract

Clusterin has been purified from ram rete testis fluid by conventional techniques and by immunoaffinity chromatography. The molecule is characterized as a glycoprotein having a molecular mass of approximately 80,000 Da and an isoelectric point of 3.6. The purified protein retains the capacity to elicit clustering of cells in an in vitro assay. Under reducing conditions in the presence of sodium dodecyl sulfate, clusterin dissociates into subunits of about 40,000 Da. Heterogeneities in apparent molecular mass were eliminated after treatment of clusterin with neuraminidase. Gel filtration chromatography revealed that clusterin exists in dimeric and tetrameric forms under conditions of neutral pH and low salt concentrations. In the presence of 6 M urea, only the monomeric form is evident, with an apparent molecular mass of approximately 85,000 Da. Clusterin, which was found to contain 4.5% glucosamine, binds to concanavalin A-Sepharose and also to wheat germ agglutinin Sepharose. The amino acid composition of clusterin is reported. The possible cellular source of clusterin in rete testis fluid is discussed. It is shown that Sertoli cells in the seminiferous tubule are one potential source, since primary cultures of rat Sertoli cells secrete a protein having the same immunochemical and physical properties as clusterin isolated from ram rete testis fluid. Possible functions of clusterin are discussed.

Published

1983

25. An objective sperm cytotoxicity assay for male-specific antisera based on ATP levels of unlysed cells: Application to assay of H-Y antigen

Author

Pierre S. Tung, Irving B. Fritz, and Robert E. Gore-Langton

Subjects

Male, endocrine system, medicine.drug_class, H-Y Antigen, Immunology, Firefly Luciferin, Monoclonal antibody, Epitopes, Mice, Adenosine Triphosphate, Antigen, medicine, Animals, Immunology and Allergy, Cytotoxic T cell, Luciferases, Cytotoxicity, Epididymis, Antiserum, biology, urogenital system, Immune Sera, Obstetrics and Gynecology, Rats, Inbred Strains, Complement System Proteins, Cytotoxicity Tests, Immunologic, Spermatozoa, Sperm, Molecular biology, Rats, Mice, Inbred C57BL, Cytolysis, Reproductive Medicine, Rats, Inbred Lew, biology.protein, Female, Rabbits, Antibody

Abstract

We correlated the decrease in levels of ATP in spermatozoa with the extent of cytotoxicity elicited by antibodies against antigenic components on sperm. In the presence of concentrations of complement which did not cause cytolysis or influence the ATP content of epididymal sperm, addition of heat-in-activated sera from non-immunized mice, rats or rabbits did not result in sperm cytolysis or a fall in ATP content. In contrast, addition of rabbit anti-rat spermatocyte sera, which has previously been shown to react with rat spermatozoa (Tung, P.S. and Fritz, I.B. (1978) Dev. Biol. 64, 297–315), did cause sperm cytolysis and a decrease in ATP content. The titre of this antiserum for 50% cytolysis was between 1:128 and 1:256, as determined by the fall in ATP content. Using these criteria, we examined the cytotoxicity against sperm of different samples of anti H-Y sera. We examined the influences of monoclonal antibody against H-Y, mouse H-Y antisera and rat H-Y antisera raised in inbred females immunized with spleen cells from males of the same strains. In all cases, anti-H-Y lowered ATP levels and lysed sperm with a cytotoxic titre between 1:8 and 1:16. Measurements of the decrease in ATP content in sperm have been shown to provide an objective and reliable estimate of the percentage of spermatozoa lysed by H-Y antisera. Cytotoxic activity of H-Y antisera was removed by absorption with spleen cells from male mice but not by absorption with spleen cells from female mice.

Published

1982

26. Changes in levels of plasminogen activator activity in normal and germ-cell-depleted testes during development

Author

Fannie E. Smith, Irving B. Fritz, and Martial Lacroix

Subjects

Male, Aging, endocrine system, medicine.medical_specialty, Phagocytosis, Biochemistry, Andrology, Plasminogen Activators, Endocrinology, Pregnancy, Spermatocytes, Internal medicine, Testis, medicine, Animals, Molecular Biology, chemistry.chemical_classification, Sertoli Cells, biology, urogenital system, biology.organism_classification, Sertoli cell, Spermatids, Spermatozoa, Protease inhibitor (biology), Rats, medicine.anatomical_structure, Enzyme, Bucladesine, chemistry, Female, Development of the gonads, Plasminogen activator, Germ cell, Bacteria, medicine.drug

Abstract

Levels of plasminogen activator activity were determined in testes obtained from normal and irradiated rats of various ages. During normal development, plasminogen activator activity per g testis increased rapidly between 40 and 60 days of age, but a comparable rise did not occur in germ-cell depleted testes of irradiated rats. Levels of enzyme in various populations of testicular cells were highest in Sertoli cells (varying between 1800 and 6300 units/mg protein in cells maintained under different culture conditions), and lowest in peritubular myoid cells (about 1 unit/mg protein), with intermediate levels in germinal cells (ranging between 147 and 560 units/mg protein in residual bodies, spermatocytes and spermatids). No protease inhibitor could be detected in germ-cell extracts. The addition to the medium in which Sertoli cells were in culture of particles which can be phagocytosed (autoclaved E. coil ) resulted in an increased formation of plasminogen activator activity by Sertoli cells. A synergistic enhancement of enzyme production resulted following the addition of submaximal quantities of dibutyryl cyclic AMP and autoclaved bacteria to Sertoli cells in culture. On the basis of these data, we suggest that the presence of advanced germinal cells during gonadal development may stimulate the synthesis of plasminogen activator by Sertoli cells, mediated in part by the phagocytosis of residual bodies by Sertoli cells which occurs prior to spermiation.

Published

1982

27. Histopathological Changes in Testes of Adult Inbred Rats Immunized Against Pachytene Spermatocytes or Sertoli Cells

Author

Pierre S. Tung and Irving B. Fritz

Subjects

endocrine system, medicine.medical_specialty, urogenital system, Somatic cell, Urology, Endocrinology, Diabetes and Metabolism, Biology, Sertoli cell, medicine.disease, Andrology, medicine.anatomical_structure, Endocrinology, Seminiferous tubule, Reproductive Medicine, Antigen, Internal medicine, medicine, Orchitis, Histopathology, Spermatogenesis, Blood–testis barrier

Abstract

Adult inbred Lewis/Wistar rats, immunized against pachytene spermatocytes or Sertoli cells prepared from maturing rats of the same strain, develop histopathological changes in the testes comparable in several respects to those reported by others in classical experimental allergic orchitis. Early changes in the structure of pachytene spermatocytes are followed by germ cell degeneration, and defoliation of germinal cells into the lumen. Concomitantly, abnormalities develop in Sertoli cell structure, and the lymph-testis barrier becomes increasingly permeable. Sertoli cells are the only testicular somatic cells which appear to be directly sensitive during the immunologic response. Disturbances in Sertoli cell functions are postulated to be crucial in the etiology of aspermatogenesis. The data are discussed in relation to the possible roles in spermatogenesis of specific antigenic determinants present on the surfaces of mature Sertoli cells and advanced germinal cells located within the adluminal compartment of the seminiferous tubule.

Published

1978

28. Stimulation by androgens of the production of androgen binding protein by cultured sertoli cells

Author

Irving B. Fritz and B G Louis

Subjects

Male, Receptors, Steroid, medicine.medical_specialty, Time Factors, medicine.drug_class, Stimulation, urologic and male genital diseases, Biochemistry, chemistry.chemical_compound, Endocrinology, Corticosterone, Internal medicine, medicine, Animals, Testosterone, Molecular Biology, Cells, Cultured, Progesterone, Androgen-binding protein, Sertoli Cells, Estradiol, biology, Dihydrotestosterone, Sertoli cell, Androgen, Androstane-3,17-diol, Rats, Kinetics, medicine.anatomical_structure, chemistry, Receptors, Androgen, biology.protein, Spermatogenesis, Androstanes, Hormone

Abstract

The formation of androgen-binding protein (ABP) by cultured Sertoli cells, prepared from testes of immature rats, is increased when androgens or follicle-stimulating hormone (FSH) are present in the medium. Testosterone and 5alpha-dihydrotestosterone are equally effective in stimulating the synthesis and secretion of ABP, but non-androgenic steroids examined (progesterone, 17beta-estradiol and corticosterone) are without influence. Maximal increases are observed when androgens are added at the time of cell plating. Cells maintained in culture medium devoid of hormones become progressively less sensitive to subsequent addition of testosterone or FSH. Data are discussed in relation to the sites of androgen requirements for spermatogenesis.

Published

1977

29. Rete Testis Fluid (RTF) Proteins: Purification and Characterization of RTF Albumin1

Author

Irving B. Fritz, Lyn Dean, Michael K. Skinner, and Kathy Karmally

Subjects

Gel electrophoresis, biology, Molecular mass, Albumin, Serum albumin, Radioimmunoassay, Cell Biology, General Medicine, Isoelectric point, Reproductive Medicine, Biochemistry, Affinity chromatography, biology.protein, Bovine serum albumin

Abstract

A major 68-kDa protein in ram rete testis fluid (RTF) is shown to be chemically and immunologically indistinguishable from albumin in ovine serum. Data obtained with two-dimensional gel electrophoresis of RTF demonstrate the presence of additional proteins with a molecular mass of 68 kDa that do not react with antisera against sheep serum albumin. Biochemical characteristics of albumin preparations isolated by immunoaffinity chromatography from ovine serum and from RTF were compared. Albumin from both sources had the same apparent molecular mass of 68 kDa, the same isoelectric point of approximately 4.2, and neither bound specifically to Concanavalin A. Analysis of tryptic peptide maps, obtained with reverse-phase high-pressure liquid chromatography, indicated no significant differences between digests of the two purified albumin preparations. Results indicate that RTF albumin and serum albumin are the same protein, which implies that RTF albumin may originate from serum. Albumin levels in RTF, collected from different rams and measured by radioimmunoassay, varied between 46 and 164 micrograms/ml, constituting between 11 and 17% of total RTF protein, while albumin levels in sheep plasma were 40,000 micrograms/ml. The protein composition of RTF is discussed in relation to the relative amounts of various components contributed by testis cells and the amounts derived from serum.

Published

1987

30. Immunolocalization of Clusterin in the Ram Testis, Rete Testis, and Excurrent Ducts1

Author

Irving B. Fritz and Pierre S. Tung

Subjects

endocrine system, medicine.medical_specialty, Clusterin, Vas deferens, Cell Biology, General Medicine, Testicle, Biology, Epididymis, eye diseases, Cell aggregation, Epithelium, Staining, Andrology, medicine.anatomical_structure, Endocrinology, Reproductive Medicine, Rete testis, Internal medicine, medicine, biology.protein, sense organs

Abstract

Clusterin, a glycoprotein that elicits cell aggregation, has previously been isolated from ram rete testis fluid, and has been partially characterized. In experiments reported, we have used monoclonal antibodies against clusterin in combination with indirect immunofluorescence microscopy to investigate the distribution of clusterin in the adult ram testis, rete testis, and excurrent ducts. Tissue blocks (5 mm3) were fixed in periodate/lysine/paraformaldehyde containing 0.1% glutaraldehyde and, after embedding, 5-microM sections were prepared for immunolocalization. In the testis, 2 basic patterns were observed: 1) strong to moderate staining for clusterin in the adluminal region with little staining in the basal region of the seminiferous epithelium and germinal cells; and 2) moderate staining throughout the seminiferous epithelium between germinal cells. In the rete testis, strong clusterin staining was localized intracellularly in the rete epithelial cells, most often associated with the luminal surface. In the epididymis, intracellular clusterin was localized in some principal cells of the caput epididymidis. The luminal surfaces and spermatozoa within the lumen were strongly positive. In the vas deferens, clusterin staining was associated with the luminal surface only. The presence of clusterin was clearly detected in unwashed isolated epididymal spermatozoa, but not in spermatozoa washed with phosphate-buffered saline containing 0.05% Tween 20.

Published

1985

31. Extracellular matrix components and testicular peritubular cells influence the rate and pattern of Sertoli cell migration in vitro

Author

Irving B. Fritz and Pierre S. Tung

Subjects

Male, endocrine system, medicine.medical_specialty, In Vitro Techniques, Biology, Extracellular matrix, Type IV collagen, Cell Movement, Laminin, Internal medicine, Testis, medicine, Animals, Molecular Biology, Cells, Cultured, Blood–testis barrier, Sertoli Cells, urogenital system, Immune Sera, Rats, Inbred Strains, Cell Biology, Sertoli cell, Extracellular Matrix, Rats, Cell biology, Fibronectin, Seminiferous tubule, medicine.anatomical_structure, Endocrinology, Microscopy, Electron, Scanning, biology.protein, Collagen, Rabbits, Type I collagen, Developmental Biology

Abstract

We report the patterns of migration of Sertoli cells plated on specific substrata, and the influences of testicular peritubular cells on these processes. Data presented indicate that while peritubular cells readily spread when explanted onto Type I collagen, Sertoli cells do not. A delay of 4 to 6 days occurs after Sertoli cells are plated before they begin to migrate randomly to form plaque-like monolayers on Type I collagen. These processes are dependent upon the synthesis and subsequent deposition of laminin and/or Type IV collagen by Sertoli cells, and are independent of fibronectin. A different behavior occurs when reconstituted mixtures of purified Sertoli cells and pertiubular cells are sparsely plated onto Type I collagen. Peritubular cells rapidly spread to form chains of cells between Sertoli cell aggregates. Sertoli cells then migrate on the surfaces of the peritubular cells, culminating in the formation of cable-like structures between aggregates. Evidence is presented that the Sertoli cell migration to form "cables" under these conditions is dependent upon fibronectin synthesized by peritubular cells, and is independent of the presence of laminin or Type IV collagen. We discuss the possible relevance of these data to the role which precursors of peritubular cells may play in determining the behavior of Sertoli cell precursors in vivo during tubulogenesis, or in the remodelling of the seminiferous tubule which occurs during different stages of the cycle of the seminiferous epithelium in spermatogenesis.

Published

1986

32. Testicular peritubular cells secrete a protein under androgen control that modulates Sertoli cell functions

Author

Irving B. Fritz and Michael K. Skinner

Subjects

Male, endocrine system, medicine.medical_specialty, medicine.drug_class, Cell, urologic and male genital diseases, Androgen-Binding Protein, Internal medicine, Testis, medicine, Animals, Testosterone, Cells, Cultured, Androgen-binding protein, Blood–testis barrier, chemistry.chemical_classification, Sertoli Cells, Multidisciplinary, Estradiol, biology, urogenital system, Transferrin, Proteins, Androgen, Sertoli cell, Culture Media, Rats, Molecular Weight, Seminiferous tubule, medicine.anatomical_structure, Endocrinology, chemistry, Androgens, biology.protein, Carrier Proteins, Research Article

Abstract

Peritubular cells of the seminiferous tubule synthesize component(s) that stimulate Sertoli cells in culture to increase the production of androgen-binding protein and testicular transferrin. The active peritubular cell component(s) are trypsin-sensitive, heat-sensitive, acid-stable molecule(s) having a molecular weight between 50,000 and 100,000. These specific factors(s) are referred to as P Mod-S to designate protein(s), produced by peritubular cells (P), that modulate the functions of Sertoli cells (S). The degree of stimulation by P Mod-S is comparable to that obtained by maximal hormonal stimulation of the synthesis of ABP and transferrin by Sertoli cells. Levels of P Mod-S secreted into the medium by primary cultures of peritubular cells are increased in the presence of testosterone. Comparable concentrations of 17 beta-estradiol do not stimulate peritubular cells to synthesize P Mod-S. Data are interpreted to indicate that androgens act on testicular peritubular cells to increase the formation of P Mod-S and that P Mod-S may modulate the properties of adjacent Sertoli cells. Findings are discussed in relation to the nature of mesenchymal-epithelial cell interactions in the seminiferous tubule and to the possible role of P Mod-S as a mediator of androgen actions of Sertoli cells.

Published

1985

33. FSH stimulation of DNA synthesis in sertoli cells in culture

Author

Michael D. Griswold, Ellen R. Mably, and Irving B. Fritz

Subjects

Male, Adenosine monophosphate, endocrine system, Cell, Biology, Biochemistry, chemistry.chemical_compound, Endocrinology, medicine, Animals, Insulin, Testosterone, Cyclic GMP, Molecular Biology, Sertoli Cells, DNA synthesis, DNA, Sertoli cell, Molecular biology, Rats, Nuclear DNA, Microscopy, Electron, Chemically defined medium, medicine.anatomical_structure, Bucladesine, chemistry, Follicle Stimulating Hormone, Thymidine

Abstract

The incorporation of [3H] thymidine into nuclear DNA was investigated in cultured Sertoli cells prepared from testes of 20-day-old rats. Addition of follicle-stimulating hormone (FSH) or dibutyryl cyclic, 3',5'-adenosine monophosphate (dbcAMP) to the culture medium greatly increased incorporation, expressed either as total amounts of [3H] thymidine incorporated per μg DNA or as the percentage of Sertoli cells with labeled nuclear DNA. No stimulation was observed in cells cultured in the presence of testosterone, insulin or cyclic 3',5'-GMP (cGMP). Light and electron microscopic autoradiographic analysis was employed to establish the identity of Sertoli cells having labeled nuclear DNA. Contaminating spermatogonia, which also took up labeled [3H] thymidine, were excluded from cell counts. In addition, Sertoli cells prepared from testes of irradiated 20-day-old germinal cell depleted rats were also observed to incorporate more [3H] thymidine into nuclear DNA when cultured in a chemically defined medium in the presence of FSH. DNA synthesis was abolished by prior treatment of cells with cytosine arabinoside. In separate experiments, the incorporation of [3H] thymidine into DNA of peritubular myoid cells was shown to be independent of FSH or dbcAMP.

Published

1976

34. Extracellular Matrix Promotes Rat Sertoli Cell Histotypic Expression In Vitro

Author

Irving B. Fritz and Pierre S. Tung

Subjects

Male, Time Factors, Cell Survival, Fluorescent Antibody Technique, Extracellular matrix, Laminin, medicine, Animals, Microscopy, Phase-Contrast, Cells, Cultured, Sertoli Cells, biology, Rats, Inbred Strains, Cell Biology, General Medicine, Seminiferous Tubules, Sertoli cell, In vitro, Extracellular Matrix, Rats, Cell biology, Fibronectin, Microscopy, Electron, Chemically defined medium, medicine.anatomical_structure, Seminiferous tubule, Reproductive Medicine, biology.protein, Ultrastructure

Abstract

We describe procedures for the preparation of a cell-free seminiferous tubule biomatrix, and provide evidence demonstrating that this material constitutes a useful substratum for maintaining the normal architecture of Sertoli cells in primary culture. Seminiferous tubule biomatrix, which has the morphological appearance of a fibrillar network rich in filaments and amorphous substance, is shown to consist of about 50% protein, most of which is collagen and glycoproteins. Fibronectin and laminin are also present in the seminiferous tubule biomatrix, as judged by immunofluorescence microscopy. Sertoli cell aggregates plated on this substratum retain a cuboidal to columnar shape, spread very slowly to form a monolayer, and survive for at least 3 weeks when cultured in a hormone-free, serum-free, chemically defined medium. In contrast, Sertoli cells plated onto uncoated polystyrene readily spread to form a monolayer of flat squamous cells which do not survive as well. Other morphological and ultrastructural characteristics are described which indicate that cells cultured on the seminiferous tubule biomatrix more closely resemble those of Sertoli cells in vivo than do cells plated on uncoated plastic. These differences in cell structure, including the maintenance of normal polarity as indicated by the presence of basolateral tight junctional complexes, remain evident for periods of 10 to 14 days after plating Sertoli cells onto biomatrix substratum. Rates of DNA synthesis by immature Sertoli cells plated onto biomatrix are less than rates by cells plated onto uncoated plastic. The data are discussed in relation to the role of substratum in the preservation of normal functions and histotype of Sertoli cells.

Published

1984

35. Cellular Localization of 5α-Reductase and 3α-Hydroxysteroid Dehydrogenase in the Seminiferous Tubule of the Rat Testis

Author

Jennifer H. Dorrington and Irving B. Fritz

Subjects

Male, endocrine system, medicine.medical_specialty, Dehydrogenase, Biology, Androsterone, chemistry.chemical_compound, Endocrinology, Spermatocytes, Internal medicine, Testis, medicine, Animals, Testosterone, Androstenedione, Hydroxysteroids, Cellular localization, Sertoli Cells, urogenital system, Age Factors, Hydroxysteroid Dehydrogenases, Dihydrotestosterone, Sertoli cell, Rats, Seminiferous tubule, medicine.anatomical_structure, chemistry, Oxidoreductases, Androstanes, medicine.drug

Abstract

Seminiferous tubules isolated from normal adult rats converted (14C) testosterone to (14C) androstanediol and (14C) androstenedione as the major metabolites; (14C) dihydrotestosterone and (14C) androsterone were produced in lesser amounts. Tubules from immature rats (26-28 days of age) converted a higher proportion of (14C) testosterone to 5alpha-reduced products than did tubules from adult rats. Spermatocyte-enriched preparations contain 5alpha-reductase. The lower level of 5alpha-reductase activity in spermatid-spermatocyte preparations indicates that this enzyme is low or absent in spermatids. Sertoli cell-enriched preparations contain 5 alpha-reductase and a high level of 3alpha-hydroxysteroid dehydrogenase. The results show that spermatocytes and Sertoli cells have the capacity to metabolise (14C) testosterone to 5alpha-reduced products; dihydrotesterone is the major product formed by spermatocytes, whereas in Sertoli cells further metabolism to 5alpha-androstane-3alpha, 17beta-diol occurs.

Published

1975

36. Steroidogenesis by Granulosa and Sertoli Cells

Author

David T. Armstrong, Jennifer H. Dorrington, and Irving B. Fritz

Subjects

endocrine system, Cell type, medicine.medical_specialty, urogenital system, Cholesterol, Urology, Endocrinology, Diabetes and Metabolism, medicine.medical_treatment, Granulosa cell, Estrone, Cleavage (embryo), Sertoli cell, Steroid, chemistry.chemical_compound, Endocrinology, medicine.anatomical_structure, Reproductive Medicine, chemistry, Internal medicine, medicine, hormones, hormone substitutes, and hormone antagonists, Hormone

Abstract

Granulosa and Sertoli cells have been isolated from the gonads of immature rats, and have been maintained in monolayer cultures in a chemically-defined medium. The hormonal requirements of these cell types for the synthesis of steroids have been studied: Granulosa cells contain cholesterol side-chain cleavage activity and synthesise progesterone when cultured in the presence of FSH and testosterone (or DHT). Sertoli cells on the other hand cannot synthesise steroids de novo. Granulosa and Sertoli cells are similar in that they are unable to convert significant amounts of progesterone to androgens. In the presence of exogenous testosterone as substrate, granulosa cells and immature Sertoli cells can synthesise estradiol and estrone when stimulated with FSH. In summary, FSH stimulates estrogen synthesis from testosterone in both cell types, and acts synergistically with testosterone (or DHT) to stimulate progesterone synthesis in granulosa cells. FSH is therefore involved in controlling the steroid environment within the gonads.

Published

1978

37. Characterization of Rat Testicular Peritubular Myoid Cells in Culture: α-Smooth Muscle Isoactin is a Specific Differentiation Marker1

Author

Irving B. Fritz and Pierre S. Tung

Subjects

biology, Cellular differentiation, Immunocytochemistry, Myoepithelial cell, Vimentin, Cell Biology, General Medicine, Sertoli cell, Molecular biology, Seminiferous tubule, medicine.anatomical_structure, Reproductive Medicine, Cell culture, Immunology, medicine, biology.protein, Immunostaining

Abstract

In frozen sections of testes from 20-day-old rats, alpha-smooth muscle (SM) isoactin was prominently immunostained in the peritubular tissue and in vascular walls, but not in areas populated by germinal cells, interstitial cells, or Sertoli cells. Peritubular myoid cell (PMC)-enriched preparations were isolated by two different procedures involving our previously published sequential enzymatic treatment ("conventional peritubular cell [PC]-enriched preparation") and by density-gradient purification of PMC from these preparations. The properties of different populations of PMC in culture were compared with respect to plating efficiency, rates of proliferation, and presence of cytoskeletal proteins. PMC, maintained in culture under defined conditions, contained proteins immunoreactive with monoclonal antibodies against alpha-SM isoactin. This was detected by immunostaining and by Western blots of cell extracts subjected to gel electrophoresis. Neither Sertoli cells, skin fibroblasts, bovine endothelial cells, nor glial cells contained alpha-SM isoactin detectable by the above techniques. We report the ontogeny of alpha-SM isoactin in the peritubular tissue of testes at different stages of gonadal development, and show that it is detectable within 8 days after birth. In addition, we describe immunocytochemical changes that occur during culture in various media of PMC prepared from testes of 20-day-old rats. We compare the use of alpha-SM isoactin as a differentiation marker for PMC with the use of desmin in facilitating the identification of PMC, and in following alterations in phenotype during culture in various culture media. Data presented demonstrate that about 81% of cells in the "conventional PC-enriched preparation," and about 94% of cells in the more purified populations of PMC were positive for alpha-SM isoactin in cells maintained in culture for 18 h after plating. These same PMC also were shown to express vimentin and plasminogen activator inhibitor, type 1. We conclude that alpha-SM isoactin is an excellent specific marker for PMC in seminiferous tubules and in culture.

Published

1989

38. Morphogenetic restructuring and formation of basement membranes by Sertoli cells and testis peritubular cells in co-culture: Inhibition of the morphogenetic cascade by cyclic AMP derivatives and by blocking direct cell contact

Author

Irving B. Fritz and Pierre S. Tung

Subjects

Male, endocrine system, medicine.medical_specialty, Cell type, Cytochalasin D, Cell Communication, Biology, Basement Membrane, chemistry.chemical_compound, Cell Movement, 1-Methyl-3-isobutylxanthine, Internal medicine, Testis, Morphogenesis, medicine, Animals, Cytoskeleton, Molecular Biology, Cells, Cultured, Blood–testis barrier, Sertoli Cells, Histocytochemistry, urogenital system, Cell Differentiation, Rats, Inbred Strains, Cell Biology, Sertoli cell, Cytochalasins, Extracellular Matrix, Rats, Cell biology, Microscopy, Electron, Endocrinology, Seminiferous tubule, medicine.anatomical_structure, Bucladesine, chemistry, Cell culture, Basal lamina, Developmental Biology

Abstract

Addition of dibutyryl cyclic AMP (dbcAMP), methylisobutylxanthine (MIX), or cytochalasin D to co-cultures of Sertoli cells and testicular peritubular myoid cells blocks a series of morphogenetic changes which otherwise occur during culture. When Sertoli cells are plated directly onto preexisting layers of peritubular cells maintained under basal conditions, structures form which display many of the characteristics of germ cell-depleted seminiferous tubules. The presence of dbcAMP, MIX, or cytochalasin D, added at varying times after plating Sertoli cells, results in the inhibition of each successive stage of in vitro remodeling: the inhibition of migration of Sertoli cells, the inhibition of initial ridge formation, the blockage of subsequent formation of mounds and nodules of compacted Sertoli cell aggregates, the prevention of the formation of basal lamina and associated layers of extracellular matrix between Sertoli cell aggregates and surrounding peritubular cells, and the inhibition of tubule formation. The presence of dbcAMP also inhibits the migration of peritubular cells, contractions by these cells, and compaction of Sertoli cell aggregates. When intimate cell apposition is prevented by plating the two cell types on either side of a membrane filter, the morphogenetic cascade is blocked, and no formation of a germ cell-depleted seminiferous tubule-like structure occurs. Other effects of dbcAMP on cell shape, cell movement, and cell association patterns during co-culture are described. Possible mechanisms by which dbcAMP, MIX, or cytochalasin D blocks restructuring are discussed. Since each elicits perturbations of the cytoskeleton, we offer the interpretation that cytoskeletal changes may be correlated with the prevention of closely apposing cell compact and the inhibition of basement membrane formation. Interactions observed between Sertoli cells and peritubular cells during co-culture are postulated to be analogous to those occurring in other types of mesenchymal cell-epithelial cell interactions during organogenesis and during tubulogenesis in the fetal testis. Speculatively, the blockage by dbcAMP of the morphogenetic cascade in the co-cultured system may be related to the inhibition by dbcAMP of testis cord formation in organ cultures of fetal gonads reported by others.

Published

1987

39. Modulation of Sertoli Cell Functions in the Two-Chamber Assembly by Peritubular Cells and Extracellular Matrix*

Author

Irving B. Fritz, Pierre S. Tung, Menachem Ailenberg, and M. Pelletier

Subjects

Male, medicine.medical_specialty, Kinetics, Biology, Diffusion, Extracellular matrix, Endocrinology, Internal medicine, Testis, medicine, Animals, Secretion, Cells, Cultured, chemistry.chemical_classification, Matrigel, Sertoli Cells, Micropore Filters, Inulin, Transferrin, Biological Transport, Rats, Inbred Strains, Sertoli cell, In vitro, Culture Media, Extracellular Matrix, Rats, Microscopy, Electron, medicine.anatomical_structure, chemistry, Cell culture, Follicle Stimulating Hormone

Abstract

A two-chamber assembly has been employed to investigate influences of peritubular cells (PC) and extracellular matrix (Matrigel) on barrier formation by Sertoli cells (SC) in culture and on transferrin production. The kinetics of transport of [3H]inulin across a Millipore filter were essentially the same in the presence or absence of Matrigel or PC. In contrast, a SC monolayer retarded the diffusion of [3H]inulin, increasing the estimated time for 50% equilibration from about 4 h to approximately 12 h. Matrigel and PC each independently further increased the equilibration time, with the largest effects elicited by the presence of Matrigel (approximately 21 h). Data have been interpreted to indicate that these two components, especially extracellular matrix, facilitate the formation of a functional barrier by SC in the two-chamber system. PC assume a more important role than Matrigel in the modulation of transferrin secretion by SC. Transferrin concentrations were higher in the inner chamber, corresponding to those in the adluminal compartment, but transferrin masses were higher in the outer chamber under the conditions described. We report the effects of the presence and absence of Matrigel, PC, and FSH on levels of transferrin secreted by SC. Addition of FSH resulted in increased transferrin secretion by SC maintained under all conditions examined. We compare our data with those previously reported by others and attempt to provide a basis for the differences observed. We discuss the properties of the system and outline major advantages and limits of the two-chamber assembly in investigations on the polarity and properties of SC in culture.

Published

1988

40. Fibronectin Synthesis is a Marker for Peritubular Cell Contaminants in Sertoli Cell-Enriched Cultures

Author

Irving B. Fritz, Pierre S. Tung, and Michael K. Skinner

Subjects

Male, endocrine system, medicine.medical_specialty, Fluorescent Antibody Technique, In Vitro Techniques, Biology, Immunofluorescence, Internal medicine, medicine, Animals, Cells, Cultured, Antiserum, Sertoli Cells, Staining and Labeling, medicine.diagnostic_test, urogenital system, Rats, Inbred Strains, Cell Biology, General Medicine, Seminiferous Tubules, Sertoli cell, Molecular biology, Fibronectins, Rats, Staining, Fibronectin, Microscopy, Electron, medicine.anatomical_structure, Endocrinology, Seminiferous tubule, Reproductive Medicine, biology.protein, Basal lamina, Antibody

Abstract

With indirect immunofluorescent microscopic techniques, we have shown that fibronectin is distributed primarily in or along the basal lamina of the seminiferous tubule boundary tissue in sections of testes from 20-day-old rats. Purified rat Sertoli cell-enriched aggregates, maintained in culture in the presence or absence of serum, exhibit no detectable immunofluorescence with fibronectin antibody, whereas purified peritubular cells in culture do have a positive reaction to fibronectin antibody. Peritubular cells in culture incorporate [35S] methionine into fibronectin which can be immunoprecipitated with a fibronectin antiserum, but Sertoli cells do not. We have used various criteria to estimate the degree of purity of Sertoli cell-enriched preparations. The presence of peritubular myoid cells in conventional Sertoli cell-enriched aggregates, cultured in the presence or absence of serum, can be detected with transmission electron microscopic examination, by the Feulgen staining procedure, and by the immunocytochemical identification of fibronectin. We describe a technique to purify Sertoli cells in conventional Sertoli cell-enriched preparations by treatment with hyaluronidase, resulting in a lesser number of peritubular cells by the above criteria, even in preparations cultured in the presence of serum. Data presented suggest that some of the products previously attributed exclusively to Sertoli cells in Sertoli cell-enriched preparations, particularly those cultured in the presence of serum, may have been contributed by peritubular cells.

Published

1984

41. Metabolic responses of Sertoli cells in culture to various concentrations of follicle stimulating hormone and cholera toxin

Author

Irving B. Fritz, Dorrington Jh, Louis Bg, and Griswold

Subjects

Male, Cholera Toxin, medicine.medical_specialty, Camp production, Stimulation, Biology, medicine.disease_cause, Follicle-stimulating hormone, Internal medicine, Cyclic AMP, medicine, Animals, Testosterone, Sertoli Cells, Estradiol, Cholera toxin, DNA, General Medicine, Sertoli cell, Rats, Kinetics, Endocrinology, medicine.anatomical_structure, Receptors, Androgen, Follicle Stimulating Hormone, Thymidine

Abstract

The concentration of cholera toxin required for half-maximal stimulation of cAMP production by Sertoli cell enriched cultures (4.48 × 10−2 μg/ml) is greater than that required for half-maximal stimulation of 17β-estradiol synthesis from testosterone (2.34 × 10−4 μg/ml), [3H]thymidine incorporation into DNA (1.48 × 10−5μg/ml), or androgen binding protein production (2.43 × 10−6 μg/ml). The same relative dose response hierarchy was obtained with respect to stimulation of Sertoli cells with follicle stimulating hormone (FSH) preparations. Again, highest concentrations were required to elicit maximal cAMP production. The data are discussed in relation to an apparent paradox: If cAMP is the mediating 'second messenger' following stimulation by FSH or cholera toxin, why should highest concentrations of these agents be required to elicit 50% of maximal cAMP levels?

Published

1978

42. Cooperativity between Sertoli Cells and Peritubular Myoid Cells in the Formation of the Basal Lamina in the Seminiferous Tubule

Author

Irving B. Fritz, Michael K. Skinner, and Pierre S. Tung

Subjects

Male, Sertoli Cells, General Neuroscience, Cooperativity, Seminiferous Tubules, Biology, Sertoli cell, Basement Membrane, General Biochemistry, Genetics and Molecular Biology, Extracellular Matrix, Fibronectins, Rats, Cell biology, medicine.anatomical_structure, Seminiferous tubule, History and Philosophy of Science, Testis, medicine, Animals, Basal lamina, Laminin, Cells, Cultured, Blood–testis barrier

Published

1984

43. Secretion of plasminogen activator by Sertoli cell enriched cultures

Author

Fannie E. Smith, Irving B. Fritz, and Martial Lacroix

Subjects

Male, endocrine system, Sertoli Cells, Lysis, urogenital system, Chemistry, Fibrinolysis, medicine.medical_treatment, Sertoli cell, Biochemistry, Cell biology, Plasminogen Activators, Tissue culture, Endocrinology, medicine.anatomical_structure, Bucladesine, Lytic cycle, medicine, Secretion, Follicle Stimulating Hormone, Molecular Biology, Plasminogen activator, Spermatogenesis, Cells, Cultured

Abstract

Conditions were established to assay plasminogen activator (PA) levels in tissue culture medium in which Sertoli cell aggregates, prepared from testes of immature rats, had been cultured. PA activity was measured by determining 125I fibrinolysis dependent upon added plasminogen. The PA levels were higher in medium taken from Sertoli cell-enriched cultures treated with follicle-stimulating hormone (FSH) or dibutyryl cAMP. In addition, the fibrin-agar overlay technique was employed to detect plasminogen-dependent lysis zones around Sertoli cell aggregates in culture. Lytic zones appeared earlier and developed faster around FSH-treated Sertoli cell aggregates. Peritubular myoid cells had no detectable PA activity when tested by either technique. The possible physiological role of PA in the testis is discussed.

Published

1977

44. Isolation and Culture of Ram Rete Testis Epithelial Cells: Structural and Biochemical Characteristics1

Author

Irving B. Fritz, Pierre S. Tung, and Joseph Rosenior

Subjects

endocrine system, medicine.medical_specialty, Cell type, Vimentin, Cell Biology, General Medicine, Biology, Testicle, Sertoli cell, Epithelium, Cell biology, Cytokeratin, medicine.anatomical_structure, Endocrinology, Reproductive Medicine, Rete testis, Cell culture, Internal medicine, medicine, biology.protein

Abstract

Cultures of rete testis epithelial cell-enriched preparations from testes of adult rams have been investigated, and some of their properties have been determined. In monolayers, the cells form mosaic-like borders, and retain many ultrastructural features characteristic of rete epithelial cells in situ, including an indented nucleus with prominent heterochromatin clumps, short rod-shaped or round mitochondria that are easily distinguished from the elongated mitochondria of Sertoli cells, the presence of desmosomes, and few if any lipid droplets or vacuoles. Unlike Sertoli cell-enriched aggregates in culture, rete testis epithelial cell preparations do not form cytoplasmic extensions, and no associated germ cells are present. Rete cells in culture express cytokeratin and vimentin in the cytoskeleton, whereas Sertoli cells prepared from testes of adult rams contain vimentin but not cytokeratin. Both rete cells and Sertoli cells stain positively for laminin but not for fibronectin, Collagen Type I, or Collagen Type III. The rete cells synthesize and secrete several proteins into the culture medium, evident in gel electrophoresis patterns of radiolabeled proteins. This pattern is similar, but not identical, to that secreted by Sertoli cell-enriched preparations. Rete cells in culture in the presence of serum continue to undergo mitotic division, but Sertoli cells do not. A variety of criteria were employed to estimate the relative numbers of Sertoli cells present in the rete testis epithelial cell-enriched preparations from testes of adult rams, including morphological and ultrastructural differences between the two cell types, and the presence of desmosomal proteins and cytokeratin in rete cells but not in Sertoli cells. The relative number of fibroblast-like cells was determined by measuring the expression of fibronectin and Collagen Type I, and an immunocytochemical probe for the detection of Factor VIII was used to estimate the degree of contamination by vascular endothelial cells. Using these markers, we determined that the rete testis epithelial cell-enriched preparations were about 93% pure. Primary cultures under defined conditions contained relatively few Sertoli cells (0.4%), but were contaminated to a larger extent by fibroblastlike cells (approximately 4%) and by endothelial cells (about 3%). The possible functions of rete testis epithelial cells are discussed herein. I NTRODU CT 10 N

Published

1987

45. Summary of the 5th European workshop on the molecular and cellular endocrinology of the testis

Author

Irving B. Fritz

Subjects

Endocrinology, Biology, Bioinformatics, Molecular Biology, Biochemistry

Published

1988

46. Interactions of Sertoli Cells with Myoid Cells in vitro

Author

Pierre S. Tung and Irving B. Fritz

Subjects

Male, endocrine system, medicine.medical_specialty, Morphogenesis, Biology, Androgen-Binding Protein, Tunica albuginea (ovaries), Internal medicine, Testis, medicine, Animals, Secretion, Cells, Cultured, Androgen-binding protein, Blood–testis barrier, Sertoli Cells, urogenital system, Cell Biology, General Medicine, Fibroblasts, Sertoli cell, Embryonic stem cell, In vitro, Rats, Cell biology, Endocrinology, medicine.anatomical_structure, Reproductive Medicine, biology.protein

Abstract

Preparations of Sertoli cells and peritubular myoid cells from testes of 20-day-old rats were cultured alone or together, and cellular interactions were assessed. In the co-cultured system, Sertoli cells within plaques became elevated, forming macroscopically visible mounds and protrusions. The morphologic characteristics of these structures were determined with scanning and transmission electron microscopy. The formation of a limiting membrane observed between individual Sertoli cell nodules and surrounding myoid cells resembled some aspects of the morphology of seminiferous tubules. Long-term co-cultures of Sertoli cells and myoid cells, stimulated by follicle stimulating hormone (FSI-l), continued to secrete androgen binding protein (ABP) under conditions in which Sertoli cell monocultures ceased production of ABP. The specificity of these cellular interactions was investigated. Bladder smooth muscle cells could substitute for peritubular myoid cells in eliciting mound formation of co-cultured Sertoli cells, but embryonic fibroblasts could not. However, embryonic fibroblasts, which did not secrete ABP, permitted FSIl-stimulated Sertoli cells in long-term co-culture to maintain ABP production. In contrast, fibroblasts from the tunica albuginea, when co-cultured with Sertoli cells, neither elicited mound formation nor supported ABP production. We conclude that while unique specificity of cellular interactions between Sertoli cells and peritubular myoid cells is not apparent in cultured preparations from testes of 20-day-old rats, these cells do retain some of the properties required for aggregation and tubule formation characteristic of tubule morphogenesis.

Published

1980

47. Identification of a non-mitogenic paracrine factor involved in mesenchymal-epithelial cell interactions between testicular peritubular cells and Sertoli cells

Author

Michael K. Skinner and Irving B. Fritz

Subjects

Male, endocrine system, medicine.medical_specialty, Mesenchyme, Cell, Cell Communication, Testicle, Biology, Biochemistry, Androgen-Binding Protein, Plasminogen Activators, Paracrine signalling, Endocrinology, FGF9, Internal medicine, Testis, medicine, Animals, Insulin, Testosterone, Growth Substances, Vitamin A, Molecular Biology, Cells, Cultured, Blood–testis barrier, Sertoli Cells, urogenital system, Transferrin, Rats, Inbred Strains, DNA, Sertoli cell, Rats, Cell biology, Molecular Weight, Testicular Hormones, Seminiferous Epithelium, medicine.anatomical_structure, Seminiferous tubule, Follicle Stimulating Hormone

Abstract

Seminiferous peritubular cells have previously been shown to secrete a protein termed P-Mod-S which modulates the functions of Sertoli cells. The present study provides an initial characterization of P-Mod-S and examines the actions of P-Mod-S on Sertoli cells. Gel filtration chromatography demonstrates that P-Mod-S has an apparent molecular weight of 70 000 that could not be dissociated to a lower molecular weight form. A 40- to 90-fold purification of P-Mod-S was obtained with a predicted half maximal effective concentration for Sertoli cells of less than 10 −9 M. Through an analysis of the actions of P-Mod-S on Sertoli cells it is demonstrated that P-Mod-S stimulates the Sertoli cell to a greater extent than any single hormone or vitamin known to influence the cell. P-Mod-S maximally stimulates testicular transferrin and androgen-binding protein production by Sertoli cells, but does not stimulate levels of plasminogen activator activity. P-Mod-S also appears to induce the synthesis of several proteins that are not detected in control non-treated Sertoli cell cultures. One such protein whose synthesis was stimulated by P-Mod-S treatment of Sertoli cells was a component having a molecular mass of 20 kDa. This 20 kDa Sertoli cell-secreted protein was specifically immunoprecipitated with an antibody against an epididymal lactalbumin-like protein. This implies that P-Mod-S can induce Sertoli cells to synthesize and secrete a lactalbumin-like protein. P-Mod-S was found not to contain mitogenic activity. Data presented indicate that testicular peritubular cells synthesize and secrete a 70 kDa non-mitogenic paracrine factor termed P-Mod-S which has a dramatic influence on Sertoli cell functions. Results are discussed with respect to modulation of epithelial (Sertoli) cell functions by components produced by mesenchymal (peritubular) cells.

Published

1986

48. Stimulation by follicle-stimulating hormone of DNA synthesis and of mitosis in cultured Sertoli cells prepared from testes of immature rats

Author

Irving B. Fritz, Michael D. Griswold, Pierre S. Tung, and Alberto J. Solari

Subjects

Male, endocrine system, medicine.medical_specialty, Mitotic index, Mitosis, Sertoli cell proliferation, Stimulation, Biology, Biochemistry, Follicle-stimulating hormone, chemistry.chemical_compound, Endocrinology, Internal medicine, Testis, medicine, Animals, Molecular Biology, Cells, Cultured, Sertoli Cells, DNA synthesis, DNA, Sertoli cell, Stimulation, Chemical, Rats, medicine.anatomical_structure, Bucladesine, chemistry, Follicle Stimulating Hormone, Thymidine

Abstract

Follicle-stimulating hormone (FSH) or dibutyryl 3',5'-cyclic AMP (dbcAMP) increases the incorporation of [ 3 H] thymidine into DNA of cultured Sertoli cells prepared from testes of rats from 4 up to 40 days of age. The amounts of DNA synthesis are shown to be inversely related to the density of the cultured Sertoli cells, and are maximal at periods 4–6 days after plating. At a given cell density the extent of DNA synthesis by primary cultures of unstimulatsd Sertoli cells is greatest in preparations from testes of rats 10 days of age or younger. The percentage of Sertoli cells capable of responding to FSH or dbcAMP with increased incorporation of thymidine into DNA becomes progressively smaller in preparations from testes of rats older than 20 days of age. The extent of DNA synthesis in Sertoli cells at different stages of development is well correlated with the percentage of cells observed to have labeled nuclei, as measured by radioautographic examination, and with the mitotic index. The frequency of mitosis of Sertoli cells, cultured in the presence of FSH, is greatest in cells prepared from testes of younger rats. Evidence is presented that the percentage of Sertoli cells which retain the capacity to undergo mitosis is reduced to nearly zero in preparations from rats older than 40 days. It is concluded that the stimulation of DNA synthesis in cultured Sertoli cells elicited by FSH or dbcAMP is directly associated with an increased mitotic frequency.

Published

1977

49. Rat Testicular Peritubular Cells in Culture Secrete an Inhibitor of Plasminogen Activator Activity1

Author

Irving B. Fritz, Pierre S. Tung, E. Balekjian, and J.A. Hettle

Subjects

Urokinase, medicine.medical_specialty, biology, Cell Biology, General Medicine, Sertoli cell, In vitro, Protease inhibitor (biology), medicine.anatomical_structure, Seminiferous tubule, Endocrinology, Reproductive Medicine, Enzyme inhibitor, Cell culture, Internal medicine, biology.protein, medicine, Plasminogen activator, medicine.drug

Abstract

Rat testicular peritubular cells in culture secrete an inhibitor of plasminogen activator (PA) activity. Conditioned serum-free medium from secondary cultures of peritubular cells (PcMEM) was concentrated and then fractionated by gel exclusion chromatography. Under native or denaturing conditions, PA inhibitor (PA-I) activity appeared in fractions having a molecular weight of approximately 55,000. The PA-I inhibited the tissuetype plasminogen activator, and also that of the two-chain form of urokinase, but not the one-chain form. Addition of guanidine HC1 (4 M) to PcMEM resulted in a large increase of inhibitory activity. The 55,000 molecular weight PA-I band in PcMEM reacted with antibodies against plasminogen activator inhibitors produced by bovine vascular endothelial cells, or by human fibrosarcoma cells, as detected by immunoadsorption experiments, by immunoblotting, and by reverse /ibrin autography. We describe other characteristics of the protease inhibitor produced by testicular peritubular cells, and we discuss its possible functions in the control of PA activity in the seminiferous tubule at different stages of spermatogenesis.

Published

1988

50. Control of Testicular Estrogen Synthesis1

Author

Irving B. Fritz, Jennifer H. Dorrington, and David T. Armstrong

Subjects

medicine.medical_specialty, Endocrinology, Reproductive Medicine, Internal medicine, medicine, Cell Biology, General Medicine, Biology, Estrogen synthesis

Published

1978