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4. Ganglioside profiles of experimental melanomas and of their melanosomal fractions

Author

Petr Hach, Borovanský J, and Eliška Vedralová

Subjects
Cancer Research, Skin Neoplasms, Cell, Melanoma, Experimental, Hamster, Dermatology, Mice, Antigen, Antigens, Neoplasm, Cricetinae, Gangliosides, medicine, Biomarkers, Tumor, Animals, G(M3) Ganglioside, neoplasms, Melanosome, Ganglioside, biology, Mesocricetus, Chemistry, Melanoma, biology.organism_classification, medicine.disease, Molecular biology, Mice, Inbred C57BL, medicine.anatomical_structure, Oncology, Mice, Inbred DBA, Melanocytes, lipids (amino acids, peptides, and proteins), Human melanoma
Abstract

We compared ganglioside profiles of animal tumours (B16 and Cloudman S91 murine melanomas, Bomirski Syrian hamster melanoma), which are widely used as models of human melanoma, and of their melanosomal fractions. A ganglioside fraction was extracted and purified and the amount of each component ganglioside was assessed by thin-layer chromatography. GM3 was the dominant ganglioside species in the murine melanomas studied. Unlike human melanomas, the GD3 expression in mouse melanomas was low. GD3 and GM3 were major gangliosides in Bomirski hamster melanoma. Alkali-labile O-acetyl-GD3, a melanoma-specific ganglioside, was detected only in Bomirski melanoma. GD2, which in human melanoma is seen as a distinct signal of tumour progression, was not found in the animal melanomas studied. Melanosomes isolated from B16 and Bomirski melanomas contained GM3 and GD3 as their major ganglioside components. These data extend the group of common antigenic determinants shared by melanosomes and cell surface of pigment cells.

Published
1995

5. Thymidine kinase in malignant melanoma

Author

Borovanský J, Netíková I, Elleder M, and Stríbrná J

Subjects
Cancer Research, Thymidine kinase activity, Melanoma, Experimental, Dermatology, Biology, Thymidine Kinase, Mice, Cytosol, Proliferating Cell Nuclear Antigen, medicine, Biomarkers, Tumor, Animals, neoplasms, Cyclophosphamide, chemistry.chemical_classification, DNA synthesis, Cell growth, Melanoma, medicine.disease, Proliferating cell nuclear antigen, Neoplasm Proteins, Specific Pathogen-Free Organisms, Isoenzymes, Mice, Inbred C57BL, Enzyme, Oncology, chemistry, Liver, Thymidine kinase, Mice, Inbred DBA, Cancer research, biology.protein, Female, Cell Division, Neoplasm Transplantation
Abstract

Thymidine kinase (EC 2.7.1.21) is an enzyme supporting DNA synthesis under conditions of increased cell proliferation. Although it has proved to be a useful marker for various malignant diseases, it has not been tested in malignant melanoma. Thymidine kinase activity was measured by means of a radioenzymic assay in two classical animal models of melanoma disease--B16 and Cloudman S91 melanoma-bearing mice. Tumour cell proliferation was assessed histochemically by measuring the expression of proliferating cell nuclear antigen (PCNA). Tumour cytosolic specific thymidine kinase activity was found to be higher in less pigmented Cloudman S91 melanoma than in differentiated, ie pigmented B16 melanoma, relative to the proliferative activity of the two tumours. Serum thymidine kinase levels were increased in melanoma-bearing animals of both types compared with healthy mice; this also reflected the efficacy of the therapy: cyclophosphamide-treated B16 melanoma-bearing mice in which the tumour development was slowed down had significantly lower serum enzyme levels in comparison with the non-treated group and the same levels compared with control, healthy mice. Our results suggest that serum thymidine kinase levels might be used as a marker to follow the effect of melanoma therapy.

Published
1994

6. Properties of melanosomes and their exploitation in the diagnosis and treatment of melanoma

Author

Borovanský J

Subjects
Male, Melanins, Cancer Research, medicine.medical_specialty, Chemistry, Melanoma, Immunotoxins, Pigment cells, Dermatology, medicine.disease, Cell biology, Melanin, Oncology, Energy absorbing, Organelle, medicine, Cytotoxic T cell, Animals, Humans, Melanocytes, Melanoma diagnosis, Melanosome
Abstract

Melanosomes are subcellular organelles with unique properties: they are producers and scavengers of cytotoxic quinones and are involved in free radical reactions. They behave as energy absorbing and converting devices, have an ion-exchange capacity and show affinity to a variety of substances. Even in the absence of melanin, premelanosomes show characteristic properties due to the presence of specific proteins. The melanosome concentration in pigment tissues is high enough to offer possibilities for influencing pigment cells and for detecting and/or killing melanoma cells. The exploitation of melanosome properties in practice is reviewed.

Published
1993

9. Isolation of melanosomes from keratinous structures: current state of the art.

Author

Borovanský, J. and Hach, P.

Abstract

Isolation of melanosomes from hair or feathers is difficult due to the need to break keratin structures using a strong chemical treatment. All recently published isolation approaches were examined in the isolation of melanosomes from human and dog hair. The best results were achieved from immediate separation of melanosomes by centrifugation after controlled NaOH hydrolysis of the hair. The crucial factor for successful separation is the choice of the optimal amount of time required for disintegration of the hair: if the time chosen is too long, melanosomes are damaged; if it is too short, contamination by residual keratin ensues. High temperatures must be avoided. Attempts to break hair structure by a number of milder reagents have failed. [ABSTRACT FROM AUTHOR]

Published
1987
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13. PP-26 Serum enzyme activities in monitoring melim melanoma progression and regression.

Author

Borovanský, J., Horák, V., Uhrová, J., Zima, T., and Elleder, M.

Subjects
*MELANOMA, *SERUM, *ENZYMES, *NEUROENDOCRINE tumors, *CANCER, *CANCER invasiveness
Abstract

Objectives of the study: To evaluate whether serum enzyme activities reflect both tumour progression and regression in a hereditary melanoma minipig MeLiM model /Cell mol Biol 45,1999,1119/ and to compare the enzyme profiles with those in murine melanomas and human disease. Material and methods: Tyrosinase activity was measured by a dopa oxidase method /Neoplasma 28,1981,59/, γ -glutamyltransferase (GGT) was monitored by means of the GGT100 set/Lachema, Czech Rep./ and neuron-specific enolase /NSE/ was analyzed with a radioimmunoassay kit /Cis-Bio Int., France/ in sera of minipigs with localized/n = 35/, metastatic /n = 22/ and cryptogenic /n = 14/ melanomas and also in animals with a spontaneous melanoma regression/n = 13/ or regression induced by devitalization therapy/n = 44/ and in control minipigs /n = 36/. Data were statistically analyzed by the Student's t -test. Results: A significant increase in tyrosinase activity (P < 0.05) was found not only in the group of animals with cryptogenic melanoma, but also in animals with spontaneous and experimentally induced melanoma regression, probably due to a better enzyme release from tumour cells. Similar results were obtained as for the GGT: There was a significant increase of activity in the groups of minipigs with regressing melanomas. NSE in experimental melanoma models has not yet been studied. The upper physiological NSE limit in minipigs (deduced as x + 2σ = 18 ng/ml) was overcome in 8 of 54 sera = in 18% of minipigs in advanced stage of melanoma progression. Conclusions: Our results document that enzyme profiles in melanoma-bearing minipigs faithfully resemble those in human counterpart (i.e. serum enzyme activities begin to be of marker value only in later stages) demonstrating that the MeLiM model is close to human melanoma unlike murine melanoma models, in which a steep increase of marker enzymes at an early stage of melanoma progression, is typical. Acknowledgements: Supported by GACR 524/01/0162 and CAV S5045113 grants. [ABSTRACT FROM AUTHOR]

Published
2003
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14. "Transcription physiology" of pigment formation in melanocytes: central role of MITF.

Author

Vachtenheim J and Borovanský J

Subjects
Animals, Base Sequence, Humans, Melanocytes cytology, Melanocytes physiology, Melanoma genetics, Melanoma physiopathology, Melanosomes physiology, Models, Biological, Promoter Regions, Genetic, Stress, Physiological, Trans-Activators genetics, Trans-Activators physiology, Melanins biosynthesis, Microphthalmia-Associated Transcription Factor genetics, Microphthalmia-Associated Transcription Factor physiology, Skin Pigmentation genetics, Skin Pigmentation physiology
Abstract

Melanin production is the primary mechanism protecting human skin against the UV light-induced damage. The polymeric compound melanin is synthesized within melanocytes in the specialized subcellular organelles, termed melanosomes, which are then transferred to surrounding keratinocytes. The genes for melanin synthesis and deposition are coordinately expressed in melanocytes. The transcription factor MITF, which has been reported to activate more than 25 genes in pigment cells, has emerged as an essential regulator not only for melanocyte development, proliferation and survival, but also for the expression of enzymes and structural proteins ensuring the production of melanin. MITF is a transcriptional activator of several genes which encode melanosome-localized proteins involved both in melanin synthesis and in melanosome biogenesis and transport, including genes whose mutations are associated with human oculocutaneous and ocular forms of albinism. Here, we outline the mechanisms of transcriptional regulation of genes associated with the biosynthesis of melanin in melanocytes and melanoma cells. MITF is crucial in this process, while several other factors seem to have only an auxiliary role to play under specific circumstances.

Published
2010
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15. SWI/SNF chromatin remodeling complex is critical for the expression of microphthalmia-associated transcription factor in melanoma cells.

Author

Vachtenheim J, Ondrusová L, and Borovanský J

Subjects
Cell Line, Tumor, DNA Helicases metabolism, Humans, Immunoprecipitation, Nuclear Proteins metabolism, Promoter Regions, Genetic, Chromatin Assembly and Disassembly, Chromosomal Proteins, Non-Histone metabolism, Gene Expression Regulation, Neoplastic, Melanoma genetics, Microphthalmia-Associated Transcription Factor genetics, Transcription Factors metabolism, Transcriptional Activation
Abstract

The microphthalmia-associated transcription factor (MITF) is required for melanocyte development, maintenance of the melanocyte-specific transcription, and survival of melanoma cells. MITF positively regulates expression of more than 25 genes in pigment cells. Recently, it has been demonstrated that expression of several MITF downstream targets requires the SWI/SNF chromatin remodeling complex, which contains one of the two catalytic subunits, Brm or Brg1. Here we show that the expression of MITF itself critically requires active SWI/SNF. In several Brm/Brg1-expressing melanoma cell lines, knockdown of Brg1 severely compromised MITF expression with a concomitant downregulation of MITF targets and decreased cell proliferation. Although Brm was able to substitute for Brg1 in maintaining MITF expression and melanoma cell proliferation, sequential knockdown of both Brm and Brg1 in 501mel cells abolished proliferation. In Brg1-null SK-MEL-5 melanoma cells, depletion of Brm alone was sufficient to abrogate MITF expression and cell proliferation. Chromatin immunoprecipitation confirmed the binding of Brg1 or Brm to the promoter of MITF. Together these results demonstrate the essential role of SWI/SNF for expression of MITF and suggest that SWI/SNF may be a promissing target in melanoma therapy.

Published
2010
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16. Microphthalmia transcription factor: a specific marker for malignant melanoma.

Author

Vachtenheim J and Borovanský J

Subjects
Biomarkers, Tumor analysis, Genetic Markers, Humans, Immunohistochemistry, Melanoma diagnosis, Microphthalmia-Associated Transcription Factor, Skin Neoplasms diagnosis, DNA-Binding Proteins analysis, Melanoma genetics, Skin Neoplasms genetics, Transcription Factors analysis
Abstract

The transcription factor microphthalmia (MITF) is required for the formation of normal melanocytes during embryonic development and for the expression of pigment cell-specific markers, which are the downstream transcriptional targets of MITF. It also seems to be crucial for the survival of malignant melanocytes. The special interest of this review is the possible utility of MITF as a marker of malignant melanoma. Melanocyte-specific isoform of MITF appears to be a unique molecule in the differential diagnosis of melanocytic tumors.

Published
2004

17. Biochemical characterization of a new melanoma model--the minipig MeLiM strain.

Author

Borovanský J, Horák V, Elleder M, Fortýn K, Smit NP, and Kolb AM

Subjects
Animals, Crosses, Genetic, Humans, Immunohistochemistry, Melanins metabolism, Melanocytes metabolism, Melanosomes metabolism, Monophenol Monooxygenase metabolism, S100 Proteins metabolism, Swine, Swine, Miniature, Ultracentrifugation, alpha-Mannosidase metabolism, gamma-Glutamyltransferase metabolism, Disease Models, Animal, Melanoma metabolism, Melanoma therapy
Abstract

Hereditary minipig melanomas, which have many histopathological and other features in common with their human counterparts, have recently become preferred melanoma models. The MeLiM (Melanoma-bearing Libĕchov Minipig) strain was selected by partial inbreeding. A high tumour incidence and malignant behaviour on the one hand together with the occurrence of spontaneous regression and high susceptibility to the devitalization technique as a new strategy in melanoma therapy, make the MeLiM strain a superior melanoma model to other hereditary swine melanomas. Biochemical analyses of the tumours revealed: (i) a high concentration of eumelanin and low concentration of phaeomelanin in melanoma cells, which makes the probability of photochemical regression of MeLiM melanomas negligible; (ii) an extremely high level of melanosomes (almost half of the melanoma dry weight), which suggests a high differentiation of the MeLiM melanoma and is consistent with its mechanical rigidity; (iii) the presence of typical melanoma enzymes--tyrosinase, alpha-mannosidase and gamma-glutamyltransferase; and (iv) in the tumours regressing as a consequence of devitalization treatment, alpha-mannosidase activity was reduced and tyrosinase activity approached the detection threshold, which is in accordance with the substitution of melanoma tissue for connective tissue in devitalized tumours observed histologically. (Immuno)histochemical comparisons (based on dopaoxidase reaction, S100 and HMB-45 reactivities) of the skin from white and pigmented minipigs revealed the absence of melanocytes in white skin. This is the first direct evidence supporting a possible explanation for the absence of melanoma in white minipigs. The similarities and dissimilarities of the MeLiM model compared with human melanoma are highlighted.

Published
2003
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18. Melanosome degradation: fact or fiction.

Author

Borovanský J and Elleder M

Subjects
Animals, Humans, Hydrolysis, Lysosomes ultrastructure, Melanins chemistry, Melanocytes metabolism, Melanoma, Experimental, Melanosomes ultrastructure, Mice, NADPH Oxidases chemistry, Oxidation-Reduction, Oxygen metabolism, Phagosomes metabolism, Polycyclic Aromatic Hydrocarbons chemistry, Spectrophotometry, Lysosomes metabolism, Melanosomes metabolism
Abstract

Our mini review summarizes what is known about the (bio)degradation of melanosomes. Unlike melanosome biogenesis where our knowledge enables us to explain it in molecular terms posing many interesting questions on the relation between lysosomes and melanosomes, melanosome degradation has remained 'terra incognita'. Observations at optical and ultrastructural levels describe the disintegration of melanosomes in the lysosomal compartment (in auto- and heterophagosomes). Histochemical studies suggest the participation of acid hydrolases in the process of melanosome degradation. Biochemical data confirm the ability of lysosomal hydrolases to degrade melanosome constituents except the melanin moiety. The similarity of melanin structure to that of polycyclic aromatic hydrocarbons suggests that melanin should be sensitive mainly, if not exclusively, to oxidative breakdown. In vitro melanin can indeed be decomposed by an oxidative attack and the degradation is accompanied by fluorescence and decreasing absorbance. From enzymes engaged in the biotransformation of polycyclic hydrocarbons only phagosomal NADPH oxidase meets the criteria (particularly as for compartmental and catalytic properties) to be involved in melanin biodegradation. The in vivo biodegradation of melanin has so far been clearly demonstrated in Aspergillus and fungi melanins.

Published
2003
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19. Autofluorescence of melanins induced by ultraviolet radiation and near ultraviolet light. A histochemical and biochemical study.

Author

Elleder M and Borovanský J

Subjects
Animals, Aorta chemistry, Fluorescence, Humans, Lipofuscin chemistry, Lipofuscin radiation effects, Paraffin Embedding, Pigment Epithelium of Eye chemistry, Pigment Epithelium of Eye cytology, Pigment Epithelium of Eye growth & development, Polymers, Skin chemistry, Skin cytology, Substantia Nigra chemistry, Substantia Nigra cytology, Immunohistochemistry methods, Melanins chemistry, Melanins radiation effects, Ultraviolet Rays
Abstract

The induction of autofluorescence of melanins by UV radiation (330-380 nm) and near UV (400-440 nm) light (jointly called UV light) was studied in tissue sections using three commercially available mounting media. Only Immu-Mount (Shandon) was found suitable for this purpose. UV irradiation of melanins in sections mounted in this medium induced strong yellow autofluorescence irrespective of the type of the polymer (eumelanin, neuromelanin, pheomelanin and ochronotic pigment). The phenomenon of autofluorescence induction was also observed with isolated natural and in vitro prepared melanins. It was inhibited by anhydrous conditions, sodium azide and catalase. In parallel experiments, rapid degradation of melanins with an intermediate fluorescent stage was achieved in UV-irradiated sections mounted in media artificially enriched with hydrogen peroxide, or directly in aqueous solutions of H2O2, Na2O2 or HIO4. Oxidations not associated with UV light led to nonfluorogenic breakdown of melanins. These observations indicate that the common mechanism may be an oxidative attack resulting from a concerted action of hydrogen peroxide and UV light leading, through strongly fluorescent intermediates, to a complete bleaching and oxidative breakdown of melanin and melanin-like polymers. Reactive oxygen species (including ozone) are considered to be important reactants in these experiments. Lipopigments differ from melanin-like pigments by their primary autofluorescence, which mostly faded during continuous prolonged irradiation. The only regular exception was melanosis coli pigment, the autofluorescence of which was considerably augmented by UV irradiation. Our results demonstrate a novel type of fluorogen in autofluorescent pigment histochemistry. The implications of the results are discussed especially in the light of the possible presence of melanin-based fluorogens in lipopigments.

Published
2001
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20. Not only fibroblasts but also melanoma cells express "leucine aminopeptidase" activity.

Author

Borovanský J, Blasko M, and Siracký J

Subjects
Cell Line, Humans, Skin cytology, Tumor Cells, Cultured, Fibroblasts enzymology, Leucyl Aminopeptidase metabolism, Melanoma enzymology
Abstract

"Leucine aminopeptidase" (LAP, aminopolypeptidase, EC 3.4.11) activity has been recommended and widely used as a histochemical marker for the identification of contaminating LAP-positive fibroblasts in pigment cell cultures. Using a sensitive biochemical assay with L-leucyl-p-nitroanilide as a substrate we demonstrated that in vitro melanoma cells also exhibit LAP activity. Our comparison of four melanoma cell lines with four fibroblast lines showed that the differences in the enzyme activity were not qualitative but only quantitative. For this reason the specific antibodies, karyological analysis and electron microscopy are recommended as more reliable means in distinguishing fibroblasts from poorly differentiated pigment cells than the LAP-cytochemistry.

Published
2000

21. Disparate behaviour of two melanosomal enzymes (alpha-mannosidase and gamma-glutamyltransferase).

Author

Borovanský J and Hach P

Subjects
Animals, Detergents pharmacology, Melanoma, Experimental enzymology, Melanoma, Experimental pathology, Melanosomes drug effects, Mice, Mice, Inbred C57BL, Neoplasm Proteins metabolism, Neoplasm Transplantation, alpha-Mannosidase, Isoenzymes metabolism, Mannosidases metabolism, Melanosomes metabolism, gamma-Glutamyltransferase metabolism
Abstract

In addition to tyrosinase and its related proteins melanosomes contain a variety of further enzyme activities. Using spectrophotometric methods alpha-mannosidase and gamma-glutamyl-transferase (GGT) were studied in B 16 melanoma, in isolated melanosomes and in tumour host (mice C57BL6J) sera. When compared to the original melanoma tissue (12.8-26.7 nkat/g TP) isolated melanosomes exhibited much higher alpha-mannosidase activity [227-420 nkat/g of total proteins (TP)]. Strong activation by Zn2+ and no influence of Co2+ ions suggested that the dominant form of alpha-mannosidase of the enzyme present in melanosomes was of the acid (lysosomal) type. The GGT activity of isolated melanosomes (168-244 nkat/g TP) was comparable with that of the whole melanoma tissue (203-375 nkat/g TP) . Treatment of melanosomes with detergents (0.1% Triton X-100, 0.5% deoxycholate) revealed striking extractibility differences between the two enzymes investigated in relation to their localization: alpha-mannosidase remained immobilized in the melanized matrix of melanosomes whereas the membrane bound GGT was easily released. Unlike the alpha-mannosidase the GGT serum levels were increasing in relation to the melanoma growth. The demonstration of acid form of alpha-mannosidase in melanosomes is consistent with their lysosomal ranking; the presence of GGT is in keeping with its expected roles both in protection against oxidative stress and in melanogenesis.

Published
1999

22. Attempts to induce melanosome degradation in vivo.

Author

Borovanský J, Hach P, Smetana K Jr, Elleder M, and Matous-Malbohan I

Subjects
Animals, Cricetinae, Dogs, Foot, Foreign-Body Reaction pathology, Granuloma pathology, Hair ultrastructure, Melanins metabolism, Melanoma, Experimental ultrastructure, Melanosomes ultrastructure, Mesocricetus, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Peritoneal Cavity pathology, Fibroblasts physiology, Lysosomes physiology, Macrophages physiology, Melanosomes metabolism, Phagocytosis
Abstract

Contradiction between repeatedly reported electron microscopic and histochemical observation of melanosome disintegration in the presence of lysosomal enzymes in vivo and failing attempts to induce such degradation by biochemical means in vitro with the aim to explain chemical mechanism(s) of this process belongs to chronically challenging problems in biochemistry of melanin structures. Attempts have been made to bring about melanosome disintegration in vivo by inoculating melanosomes isolated from dog hair into the tissue of amelanotic Bomirski melanoma and into peritoneal cavities of DBA/2 and C57BL/6J mice, and by repeated injection of melanosomes isolated from Bomirski pigmented melanoma into Syrian hamster foot pads. Both histological and electron microscopic observations demonstrated that melanosomes were phagocytized by macrophages and sporadically by fibroblasts. In peritoneal cavities the injected foreign melanosomes remained mostly extracellularly, were surrounded by foreign body multinuclear cells and formed granulomas. There were no convincing signs of degradation of the hair melanosomes, which behaved like inert foreign bodies. Only some phagocytized Bomirski hamster melanoma melanosomes tended to lose their integrity. Our data suggest that melanosomes devoid of their limiting membranes are not necessarily prone to extensive disintegration in vivo. The earlier reported association of lysosomal enzymes with disintegrating melanosomes does not constitute an evidence for their participation in melanosome degradation. Considering the structure of melanins, redox mechanisms (analogous with the metabolism of polycyclic hydrocarbons (DePierre and Ernster, 1978)) seem to be more probably involved in pigment degradation than hydrolytic reactions.

Published
1999

23. Tumour tissue is a source of gamma-glutamyl transpeptidase sialoform in the sera of melanoma-bearing mice.

Author

Melezínek I, Borovanský J, Elleder M, and Bubnová E

Subjects
Animals, Chromatography, Ion Exchange, Electrophoresis, Polyacrylamide Gel, Female, Isoenzymes drug effects, Isoenzymes isolation & purification, Liver enzymology, Melanoma, Experimental blood, Melanoma, Experimental pathology, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Molecular Weight, Neuraminidase pharmacology, gamma-Glutamyltransferase drug effects, gamma-Glutamyltransferase isolation & purification, Isoenzymes metabolism, Melanoma, Experimental enzymology, N-Acetylneuraminic Acid metabolism, gamma-Glutamyltransferase metabolism
Abstract

The total serum activity of gamma-glutamyl transpeptidase (GGT) was shown to increase with the growth of transplantable B16 and S91 melanomas in inbred mice. In an effort to define the source of the GGT shed into the bloodstream the physicochemical characteristics of the partially purified GGT isoforms from liver, serum and B16 melanoma were compared. The molecular weights of the serum and melanoma isoforms were identical (86 kDa) and differed from that of the liver isoform (69 kDa). In polyacrylamide gel electrophoresis the serum and melanoma isoforms had a similar mobility which exceeded that of the liver enzyme. Treatment of the enzyme preparations with neuraminidase removed the differences in the electrophoretic mobility of the three GGT isoforms studied. On ion exchange chromatography on a DEAE-Spheron 300 LC column the melanoma and serum isoforms had an affinity to the sorbent unlike the liver isoform. Our observations suggest that melanoma cells express a sialoform of GGT which is responsible for an increase in the total GGT serum activity. Biochemical and histochemical analyses did not reveal any increase in liver GGT production associated with melanoma development. Detection of the GGT isoform of tumour origin in sera ranks GGT among the specific melanoma markers.

Published
1998

24. Cytotoxic interactions of Zn2+ in vitro: melanoma cells are more susceptible than melanocytes.

Author

Borovanský J, Blasko M, Siracký J, Schothorst AA, Smit NP, and Pavel S

Subjects
Chelating Agents pharmacology, Drug Screening Assays, Antitumor, Edetic Acid pharmacology, Humans, Melanocytes cytology, Melanoma pathology, Tetracycline pharmacology, Tumor Cells, Cultured drug effects, Zinc pharmacokinetics, Melanocytes drug effects, Melanoma drug therapy, Zinc pharmacology
Abstract

Previous studies have shown that sensitivity to high extracellular levels of Zn2+ is a general feature of cells in vitro and that a prerequisite of the toxic action of zinc is entry into cells via channels that are shared with iron or calcium. As the biochemical and toxicological behaviour of zinc chelate complexes could be different from that of free Zn2+, the effect of chelating agents on zinc transport into human melanoma cell lines was tested. EDTAcal and tetracycline reduced the toxic action of zinc ions in vitro, whereas phenytoin and diethyldithiocarbamate potentiated its effects. D-penicillamine, an effective chelator of zinc in vivo, also exerted a protective action in vitro. Comparison of sensitivity to Zn2+ in vitro between human melanoma lines and several lines of pigment cells from skin of various origins demonstrated that melanoma cells are killed by zinc ions at concentrations which are only partially toxic for normal pigment cells. This is consistent with the repeatedly observed high uptake of 65Zn by melanoma cells.

Published
1997
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25. Detection of metals in tissues, cells and subcellular organelles.

Author

Borovanský J

Subjects
Animals, Humans, Metals analysis
Abstract

The current state of art in the detection of metals in tissues, cells and their subcellular fractions has been reviewed. Both classic chemical techniques (including titration, spectrophotometric, electrochemical and isotope methods, neutron activation analysis, mass spectrometry, inductively coupled plasma) and cell biology techniques (i.e. conventional histochemical methods, autometallography, autoradiography and microanalytical techniques using beam of electrons or protons, laser, X-ray or ion beam) were discussed. This survey of analytical techniques is, wherever possible, illustrated by examples documenting how our knowledge on metals in pigment cells and their subcellular fractions has been growing.

Published
1997

26. Experimental chemotherapy of murine melanomas: is there a discrepancy compared to clinical experience?

Author

Borovanský J

Subjects
Animals, Antineoplastic Agents administration & dosage, Biomarkers, Tumor blood, Melanoma enzymology, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Neoplasms, Experimental drug therapy, Neoplasms, Experimental enzymology, Survival Rate, gamma-Glutamyltransferase blood, Antineoplastic Agents therapeutic use, Melanoma drug therapy
Abstract

There has been a discrepancy between promising results of experimental chemotherapy in animal melanoma models and clinical response rates. This inconsistency seems to reflect weak points of the assays used so far to monitor the response of melanoma cells to chemotherapeutic agents. Therefore a less usual approach was chosen in the present study: Tumor cells were cultured in peritoneal cavity (B16 melanoma in inbred C57BL/6J mice and Cloudman S91 melanoma in inbred DBA2 mice) to maintain normal in vivo conditions; the animals were receiving the tested agents in i.p. injections and the prolongation of their life span was considered as the principle parameter of therapeutic efficiency of the compounds tested. Previously described therapeutic potency both of vitamins (C, alpha-tocopherol acid succinate) and some phenols (hydroquinone, 4-hydroxyanisole) was confirmed. Benzoate, spin trap N-butyl-alpha-phenyl-nitrone and ammonium chloride as a lysosomotropic agent failed to increase the survival of melanoma-bearing mice. Free radical scavenger methimazole exerted a therapeutic effect in mice with pigmented B16 melanoma. Only classic cytostatic agents--cisplatin and cyclophosphamide--proved its therapeutic effect in both melanoma models studied. These results are in accord with the known resistance of human melanoma to conventional chemotherapy. Measurement of serum activity of gamma-glutamyltransferase was shown to be useful for monitoring therapeutic effect.

Published
1997

27. Free radical activity of melanins and related substances: biochemical and pathobiochemical aspects.

Author

Borovanský J

Subjects
Animals, Humans, Indoles metabolism, Lipofuscin metabolism, Melanins chemistry, Melanins metabolism, Melanocytes metabolism, Free Radicals metabolism, Melanins biosynthesis
Abstract

Human body contains a number of natural pigments-authentic melanins, soluble melanins, neuromelanins, lipofuscins-having a similar origin-oxidation and polymerization of precursor phenols, and sharing many common characteristics among which dominates their free radical activity. Related substances can be formed from exogenous compounds introduced at some occasions to the organism. The functional properties of the pigments seem to be determined by their localization, i.e. cellular or extracellular, and as regards those intracellular ones by their subcellular compartmentalization. All the intracellular pigments mentioned in this study are associated with lysosomal enzymes at some stage of their development. A special attention was paid to a neglected group of soluble melanins. It was proposed that methylation may decide about the fate of precursor molecules whether they will join the soluble melanin pool or will be excreted as melanogens. Participation of the pigments in various biochemical and pathobiochemical processes has been reviewed.

Published
1996

28. Approaches to prove the melanoma origin in amelanotic human melanoma cell lines.

Author

Blasko M, Chalupa I, Borovanský J, Toceková M, and Siracký J

Subjects
DNA, Neoplasm analysis, Female, Humans, Karyotyping, Melanoma, Amelanotic enzymology, Melanoma, Amelanotic genetics, Middle Aged, Reproducibility of Results, Skin Neoplasms enzymology, Skin Neoplasms genetics, Tumor Cells, Cultured enzymology, Melanoma, Amelanotic pathology, Skin Neoplasms pathology, Tumor Cells, Cultured pathology
Abstract

The human melanoma B-HM8 cell line was derived from highly pigmented malignant skin melanoma. After 5 weeks of cultivation it entirely lost the pigmentation and has remained amelanotic since. Electron microscopy revealed neither premelanosomes nor melanosomes and the cells did not release detectable amount of dopa-oxidase activity into culture medium. Immunocytochemical studies using the polyclonal anti-S-100 antibody and detection of alpha-mannosidase activity in culture medium proved the melanoma origin of B-HM8 cells. Chromosomal changes in the karyotype of these cells were typical for human melanoma with chromosomes No. 1, 5, 7, 9, and 11 involved most frequently.

Published
1996

29. Evaluation of serum sialic acid fractions as markers for malignant melanoma.

Author

Vedralová E and Borovanský J

Subjects
Animals, Biomarkers, Tumor, Cricetinae, Mesocricetus, N-Acetylneuraminic Acid, Neoplasm Transplantation, Melanoma blood, Sialic Acids blood
Abstract

Increased total serum sialic acid levels have proved to be a useful non-specific marker of various neoplastic diseases including melanoma. In some malignancies, specific fractions of sialic acid were reported to be more reliable for monitoring disease progression. In this study various fractions of sialic acid were measured in the sera of Bomirski melanoma-bearing Syrian hamsters using the modified thiobarbituric acid method of Skoza and Mohos. Significantly higher serum levels of total sialic acid, 601.0 +/- 49.1 micrograms/ml, were demonstrated in animals with melanoma in comparison with control hamsters, 463.1 +/- 33.0 micrograms/ml (P < 0.01). Free sialic acid concentration was found to be negligible compared with that found in the sera of melanoma patients. Lipid bound sialic acid measurements carried out according to Bhatavdekar et al. were shown to be influenced by interfering substances. Hence, only the estimation of total sialic acid in sera can be recommended for monitoring melanoma progression. Bomirski melanoma proved to be a good model of human melanoma.

Published
1994
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30. Zinc in pigmented cells and structures, interactions and possible roles.

Author

Borovanský J

Subjects
Animals, Humans, Ligands, Melanins metabolism, Melanocytes metabolism, Melanoma metabolism, Metallothionein metabolism, Pigmentation physiology, Zinc metabolism
Abstract

Zinc is a feature trace element of pigment cells and tissues. Organelles, in which melanin is synthesized and stored, i.e. melanosomes, represent a zinc reservoir at the subcellular level. In order to understand function of metals in tissues, cells and their constituents, knowledge is needed on metal interactions with intracellular targets. The possible zinc ligands in pigment cells include melanin, metallothionein, melanotransferrin, B700 and related proteins, ferritin, zinc enzymes and low molecular weight ligands. Areas of a special interest in relation of pigment cells and structures to zinc--such as zinc effect on melanogenesis, zinc excretion and buffering by melanosomes, zinc function in free radical processes as well as zinc role in melanomas--have been reviewed. High level of zinc in pigment cells may indicate a physiological defense against the potential danger of oxidative stress.

Published
1994

31. Morphometric parameters of isolated melanosomes.

Author

Hach P, Borovanský J, and Vedralová E

Subjects
Animals, Cell Separation, Cricetinae, Microscopy, Electron, Eye cytology, Hair cytology, Melanocytes ultrastructure, Mesocricetus anatomy & histology, Mice anatomy & histology
Abstract

Basic morphometric parameters of melanosomes isolated from mouse hair, hamster eye and hamster hair are given and tabelized with those published formerly to enlarge the widest published collection of melanosomes isolated from different types of pigmented tissues up to 17 types. The splitting of melanosomes isolated from mixed tissue of hamster eyes into two subpopulations confirmed the presence of double origin of melanosomes in the eye. The close correspondence of subpopulations of hamster eye melanosomes with hamster hair and hamster melanoma (type Bomirski) respectively supports the hypothesis of high structural stability of melanosomes even under pathological conditions.

Published
1993

32. Melanosome--a sophisticated organelle.

Author

Hach P, Borovanský J, and Vedralová E

Subjects
Animals, Humans, Melanins metabolism, Melanocytes physiology, Melanocytes ultrastructure
Abstract

Melanosome is a clear out organelle of its own. The experience of the authors in the melanosome investigation has been reviewed and put to context with the literature data. Melanin moiety, a prominent feature of melanosome, was found to vary between 20-60 weight %. Melanosome concentration in pigment tissues was demonstrated to be remarkably high which explains their capacity to perform various functions both cytoprotective and cytotoxic-ascribed to the presence of melanin. Putative relation of melanosomes to other cell organelles was critically analysed. Systems of melanosome maturation were explained. The ultrastructure of melanosomes determined by the quality of their protein matrix was described and basic morphometric data summarized. The importance of the compartmentalization of melanogenesis was underlined and the fragility of melanosomal limiting membrane shown. The melanosome degradation repeatedly observed by electron microscopy has not been confirmed by biochemical means.

Published
1993

33. An estimate of melanosome concentration in pigment tissues.

Author

Borovanský J, Vedralová E, and Hach P

Subjects
Animals, Cattle, Cricetinae, Decapodiformes cytology, Dogs, Hair cytology, Horses, Humans, Ink, Melanoma pathology, Mesocricetus, Mice, Melanocytes, Pigments, Biological
Abstract

Concentration of melanosomes in various tissues has been unknown because of the impracticability of their direct quantification. Using an indirect approach comprising the estimation of melanin both in freeze-dried tissue samples and in isolated melanosomes, we obtained data on the amount of melanosomes in various pigment tissues. The concentrations of melanosomes found in the tissues were relatively high, not only reflecting the dark color of pigment tissues but also explaining their capacity to perform various functions ascribed to the presence of melanin.

Published
1991
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34. Possible relationship between abnormal melanosome structure and cytotoxic phenomena in malignant melanoma.

Author

Borovanský J, Mirejovský P, and Riley PA

Subjects
Animals, Brain Neoplasms metabolism, Brain Neoplasms pathology, Brain Neoplasms secondary, Cell Membrane pathology, Female, Humans, Melanoma secondary, Mice, Mice, Inbred C57BL, Microscopy, Electron, Neoplasm Transplantation, Skin Neoplasms metabolism, Skin Neoplasms pathology, Vaginal Neoplasms metabolism, Vaginal Neoplasms pathology, Lipid Peroxidation, Liver metabolism, Melanocytes pathology, Melanoma metabolism, Melanoma pathology
Abstract

Melanogenesis has been regarded as a hazard for pigment cells which are endangered by reactive quinones and semiquinones generated by this process. Normally the potentially cytotoxic species are confined to melanosomes by a limiting membrane and thus separated from the rest of the cell. Our electron microscopic investigation has demonstrated the presence of abnormal and incomplete melanosomes in human melanomas from epidermal and mucosal sites, in melanoma metastases, and in B16 mouse melanoma. We conclude that significant leakage of reactive melanin precursors including free radical species may occur from aberrant melanosomes in pigmented tumors. This would be expected to be reflected by fully extended physiological scavenging mechanisms, and by local and distant manifestations of cytotoxicity: Among these manifestations is free radical damage to the liver, detected by a thiobarbituric acid-reactive substances assay, in B16 melanoma-bearing mice. The efflux of toxic species from abnormal melanosomes may explain both the observed frequent occurrence of necrosis in melanomas and the therapeutic efficacy of tyrosinase substrates and may also be one of the factors influencing the extent of melanogenuria.

Published
1991

35. [Melanosomes from the biochemical viewpoint].

Author

Borovanský J

Subjects
Animals, Carbohydrates analysis, Cattle, Guinea Pigs, Lipids analysis, Melanins analysis, Melanocytes analysis, Melanocytes enzymology, Mice, Nucleic Acids analysis, Proteins analysis, Melanocytes metabolism
Published
1979

36. Enzyme histochemistry of human melanomas and pigmented naevi with special reference to alpha-D-mannosidase activity.

Author

Elleder M, Borovanský J, Mazánek J, and Vosmík F

Subjects
Acid Phosphatase analysis, Alkaline Phosphatase analysis, Carboxylesterase, Carboxylic Ester Hydrolases analysis, Glucuronidase analysis, Histocytochemistry, Humans, Monophenol Monooxygenase analysis, Oxidoreductases analysis, alpha-Mannosidase, Mannosidases analysis, Melanoma analysis, Nevus, Pigmented analysis, Skin Neoplasms analysis
Abstract

A histochemical study of alpha-D-mannosidase revealed that normal human melanocytes (resting state, activated, lentigo simplex) exhibit either no or just detectable activity, as do melanocytes in the initial phase of lentigo maligna. Junctional, or occasionally zone A naevocytes displayed a very low enzyme activity. On the other hand, melanocytes in the initial stage of neoplastic transformation (dysplastic naevi, advanced stage of lentigo maligna) and also melanoma cells in disorders of low malignant potential (initial naevogenic melanoma, superficial spreading melanoma) displayed a high activity uniformly throughout the cell population. In the malignant forms (nodular melanoma, recurrences, metastases), the enzyme activity was remarkably heterogeneous, suggesting a breakdown of uniformity during malignant transformation. The significance of alpha-mannosidase activity induction in the course of melanocyte neoplastic transformation is not clear at present. The results of biochemical assays suggest that the lysosomal isoenzyme is mainly responsible. Other lysosomal enzymes, and dehydrogenases studied concomitantly, did not display any comparable phenomena of induction or similar behaviour. However, the results of a comparison of alpha-mannosidase with the melanocyte reference enzyme tyrosinase suggested activity patterns in the enzyme pair which may provide a better insight into the biochemical differentiation of human melanocytes in neoplastic disorders. The possible relationship of alpha-mannosidase to melanogenesis is also discussed.

Published
1986
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37. Soluble melanoprotein of tumor origin.

Author

Borovanský J, Hach P, and Duchon J

Subjects
Female, Humans, Neoplasm Proteins analysis, Solubility, Melanoma analysis, Neoplasm Proteins isolation & purification, Skin Neoplasms analysis
Abstract

The procedure for isolating soluble melanoprotein from human malignant melanoma was described. Electron microscopy confirmed the absence of any contaminating organized particles. The melanoprotein was brown hygroscopic substance with 8.8% of melanin, easily soluble in water. The solution revealed general absorption with a shoulder at 280 nm. Chemical composition was typical for a melanoprotein complex with characteristic high sulphur content (2.1%) and abundance in zinc (210 mug Zn/g dry sample). Sedimentation and electrophoretic properties indicated relative homogeneity. Similar substance could also be isolated from Harding-Passey mouse melanoma. Such soluble melanoproteins have been needed for their broad exploitation in tumor immunology.

Published
1975

38. Parameters of melanoma differentiation.

Author

Borovanský J, Elleder M, and Hach P

Subjects
Animals, Cricetinae, Histocytochemistry, Humans, Melanoma enzymology, Monophenol Monooxygenase metabolism, Melanins metabolism, Melanoma metabolism
Published
1980

40. Human melanoma cell lines: morphology, growth, and alpha-mannosidase characteristics.

Author

Siracký J, Blasko M, Borovanský J, Kovarík J, Svec J, and Vrba M

Subjects
Cell Line, Female, Humans, Melanoma enzymology, Middle Aged, Monophenol Monooxygenase analysis, Mannosidases analysis, Melanoma pathology
Abstract

Four human melanoma cell lines were characterized by evaluation of the morphology, ultrastructure, cytogenetics, plating efficiency, agar colony formation and alpha-mannosidase values. Biochemical studies demonstrate that all studied lines produced alpha-mannosidase even under condition of long-term in vitro growth. All respective lines were characterized by a great variations in biological markers studied and very few reliable comparisons could be obtained as regards the proliferation activity and capacity, cellular composition and clonogenic potential as well. Due to cellular selections during long-term in vitro cultivation, the range for using these experimental systems as models for the study of biology of human malignant melanoma seems to be rather limited.

Published
1982

41. The hair melanosome: another tissue reservoir of zinc.

Author

Borovanský J, Horcicko J, and Duchon J

Subjects
Animals, Cell Fractionation, Copper analysis, Cytoplasmic Granules analysis, Dogs, Female, Hair analysis, Humans, Male, Hair ultrastructure, Melanocytes ultrastructure, Zinc analysis
Abstract

Melanosomes were isolated from human and dog hairs and their Zn content was determined. The mean Zn concentrations, in mug Zn/g dry weight, were 687 (men's melanosomes), 641 (women's melanosomes) and 691 (dog melanosomes). These values rank melanosomes from pigmented keratinous structures among the structural elements with the highest Zn content. An interpretation of the possible causes of this accumulation was submitted. By means of the conversion factor between hair length and weight (determined at 0.004), it was estimated that daily Zn lossess via hair vary in the region of 19 mug. In detailed studies of Zn metabolism, excretion via pigmented keratinous structures ought not to be neglected.

Published
1976

43. Chromatographic separation of melanosomes.

Author

Borovanský J, Hach P, and Duchon J

Subjects
Animals, Cattle, Cell Fractionation methods, Chromatography, Gel, Eye ultrastructure, Hair ultrastructure, Humans, Mice, Microscopy, Electron, Neoplasms, Experimental ultrastructure, Organoids ultrastructure, Melanocytes ultrastructure, Melanoma ultrastructure
Published
1977
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45. Quantitative parameters of melanomas differentiation.

Author

Borovanský J

Subjects
Animals, Cattle, Cell Differentiation, Cricetinae, Dogs, Hair analysis, Horses, Humans, Melanoma pathology, Mice, Neoplasms, Experimental analysis, Pigment Epithelium of Eye analysis, Pigmentation, Substantia Nigra analysis, Melanins analysis, Melanoma analysis
Abstract

Melanin concentration which represents one of biochemical parameters expressing the degree of pigment cell differentiation was studied by new gravimetric procedure in human, Bomirski hamster, Harding-Passey mouse and horse melanomas and also in several non-tumor pigment tissues. In amelanotic varieties of human and hamster melanomas relatively high melanin level was discovered. This finding (together with known electron microscopic evidence of pre-melanosomes presence in some amelanotic melanomas) suggests that the term "amelanotic" is not correct. Comparison of melanin content between melanomas and normal pigment tissues clearly demonstrates in quantitative way that as for melanomas their proliferation does not decrease the degree of their biochemical differentiation.

Published
1978

46. The effect of zinc on mouse melanoma growth in vitro and in vivo.

Author

Borovanský J, Riley PA, Vránková E, and Necas E

Subjects
Animals, Cell Division drug effects, Cell Line, Diet, Melanoma pathology, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Zinc pharmacology, Melanoma metabolism, Zinc metabolism
Abstract

The effect of Zn2+ on mouse melanoma growth in vitro and in vivo was studied. Under in vitro conditions the proliferation of a Cloudman mouse melanoma cell line was inhibited by zinc ions at 10(-4) M, as measured by 3H-thymidine incorporation and optical density of NaOH cell digests. However, in vivo it was not possible to suppress both B16 and Cloudman S91 melanoma growth in mice by the administration of zinc ions. There were no significant differences in tumor growth after subcutaneous inoculation between mice constantly receiving 0.1% zinc acetate or 0.05% zinc sulphate in their drinking water and control groups, nor was it possible to decrease the number of lung metastases by zinc treatment after intravenous inoculation of tumor cells. The increased dietary supply of Zn failed to influence the survival time of mice in both melanoma types studied. Preincubation in vitro of cell suspensions in 10(-3) M zinc acetate prior to injection inhibited melanoma development in vivo. This implies that the in vivo zinc levels did not reach the necessary cytotoxic concentration.

Published
1985

47. Ultrastructural and biochemical characteristics of isolated melanosomes.

Author

Hach P, Duchoń J, and Borovanský J

Subjects
Animals, Cattle, Chick Embryo, Cytoplasmic Granules analysis, Cytoplasmic Granules ultrastructure, Dogs, Humans, Melanins analysis, Melanocytes analysis, Mollusca ultrastructure, Proteins analysis, Melanocytes ultrastructure
Published
1977

49. Cytotoxicity of zinc in vitro.

Author

Borovanský J and Riley PA

Subjects
Animals, Biological Transport, Cell Division drug effects, Cell Line, HeLa Cells cytology, HeLa Cells drug effects, Humans, Melanoma, Experimental, Zinc metabolism, Cell Survival drug effects, Zinc pharmacology
Abstract

The effect of zinc ions on B16 mouse melanoma lines, HeLa cells and I-221 epithelial cells was investigated in vitro in order to ascertain whether sensitivity to Zn2+ is a general feature of cells in vitro and in an attempt to elucidate the mechanism(s) of zinc cytotoxicity. The proliferation of B16, HeLa and I-221 cell lines was inhibited by 1.25 x 10(-4), 1.50 x 10(-4) and 1.50 x 10(-4) mol/l Zn2+, respectively. The free radical scavengers, methimazole and ethanol, did not suppress the toxicity of Zn2+, neither did superoxide dismutase or catalase. The addition of the chelating agent EDTA reduced the zinc cytotoxicity. It was possible to suppress the cytotoxicity of zinc by increasing the concentration of either Fe2+ or Ca2+ but not Mg2+, which suggests that a prerequisite for the toxic action of zinc is entry into cells using channels that are shared with iron or calcium. This view was supported by experiments in which transferrin intensified the cytotoxic action of zinc in serum-free medium. Another agent facilitating zinc transport, prostaglandin E2, inhibited the proliferation of the B16 melanoma cell line. There were no conspicuous differences in zinc toxicity to pigmented and unpigmented cells. The toxic effect of zinc in the cell systems studied exceeded that of iron, copper, manganese and cobalt in the same concentration range. In vitro, Zn2+ should be regarded as a dangerous cation.

Published
1989
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50. Excretion of melanogens and zinc during the growth of melanoma in hamsters.

Author

Horcicko J, Pavel S, Borovanský J, and Duchon J

Subjects
Animals, Creatinine urine, Cricetinae, Magnesium urine, Male, Neoplasm Transplantation, Neoplasms, Experimental urine, Transplantation, Homologous, Melanins urine, Melanoma urine, Zinc urine
Abstract

Melanogens which are considered as probable precursors or their metabolites in the metabolic pathway toward melanin are excreted in an increasing amount during the melanotic melanoma growth in hamsters. Moreover, an increased excretion of zinc was observed. The evaluation of dependence between zinc and Thormählen positive melanogens excretions during the melanoma growth suggests an exponential type of dependence. Likewise as in the case of human melanoma the hyperzincuria proved to be a laboratory sign of tumor disease progression in Syrian hamsters as well. The cause of an increased zinc excretion during the melanoma growth seems to consist in an increased lysis of pigment cells. The presumed destruction of tumor cells was not accompanied by a higher excretion of magnesium, though. Concentration of creatinine proved to be a useful mean for expressing of standard excretion of various substances also in hamsters.

Published
1979

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