Your search keyword '"Aaron E. Freeman"' showing total 25 results

1. Characterization of mouse fetal lung cells cultured on a pigskin substrate

Author

Christopher Hassett, Paulette Melfi, Michael J. Byers, Yutaka Yoshida, Aaron E. Freeman, and Virginia Hilborn

Subjects

Swine, Bronchi, Plant Science, Biology, Matrix (biology), Mice, Dermis, Culture Techniques, Precursor cell, Organoid, medicine, Animals, Lung, Skin, Mucin, Esterases, gamma-Glutamyltransferase, Alkaline Phosphatase, Molecular biology, Organoids, Pulmonary Alveoli, medicine.anatomical_structure, Biochemistry, Alkaline phosphatase, Immunohistochemistry, Cell Division, Biotechnology

Abstract

Lung organ bits taken from full-term mice were explanted on the dermal surface of sterile, dead pigskin. The cells migrated onto the pigskin dermis and proliferated to form an organoid culture consisting of ductular structures separated by a matrix of epithelial cells. Cells within the ductular structures were ciliated, produced mucin, and exhibited the activities of nonspecific esterase and gamma-glutamyl transferase; therefore they were considered to be derived from bronchial epithelium. Cells forming the matrix possessed the activities of nonspecific esterase and alkaline phosphatase and contained lamellar structures typical of surfactant-producing pneumocyte Type II cells; therefore they were considered to be derived from alveolar precursor cells.

Published

1980

2. Carcinogenesis in vitro

Author

Aaron E. Freeman, Paul J. Price, and Howard J. Igel

Subjects

biology, Contact inhibition, Endogeny, Embryo, Plant Science, biology.organism_classification, Virology, Molecular biology, Virus, Transformation (genetics), Cell culture, Murine leukemia virus, Ploidy, Biotechnology

Abstract

SUMMARY Susceptibility to chemically induced transformation changed as a rat embryo cell culture was passaged. For the first 35 to 60 passages, the cultures were diploid and resistant to transformation by chemical carcinogens. However, cultures infected with a murine leukemia virus were transformed by chemicals. For the next 60 passages, the cultures were heteroploid, but retained contact inhibition and were not tumorigenic. Even without addition of heterotypic viruses, these heteroploid cultures could be transformed by chemicals, but the endogenous rat C-type virus could be demonstrated in the transformed cultures. At higher passages, the rates of spontaneous transformation gradually increased so that the cultures could not be used for transformation studies. Chemically induced transformation of the stable heteroploid cell line (F1706) was manifested by an easy to read focal alteration. Initial observations based on these foci were confirmed by inoculating the morphologically altered cells into isogeneic newborn rats.

Published

1975

3. Fine structural identification of organoid mouse lung cells cultured on a pigskin substrate

Author

Virginia Hilborn, Yutaka Yoshida, and Aaron E. Freeman

Subjects

Cell type, Cellular differentiation, Type-II Pneumocytes, Explanted Organ, Cell Differentiation, Plant Science, Biology, Lamellar granule, Cell biology, Extracellular matrix, Mice, Microscopy, Electron, Organ Culture Techniques, Ultrastructure, Organoid, Animals, Cilia, Lung, Biotechnology

Abstract

Mouse full-term embryonic lung tissue was cultured as organ bits using dead, sterile pigskin dermal collagen as a substrate. Explanted organ bits grew on the surface of, and into, the pigskin dermal collagen for at least 9 weeks after the initiation of culture. The outgrowth consisted of a thick cellular sheet containing various sizes of ductular structures within a cellular matrix that did not show any particular structure. Electron microscopic observation revealed that the larger ductular structures consisted largely of ciliated cells. The smaller ductular structure consisted largely of Type II pneumocytes containing lamellar bodies. The cellular matrix consisted of Type II pneumonocytes and other cell types including fibroblasts and macrophages in the early stage of cultivation. Macrophages invaded the pigskin dermal collagen. An intermediate cell type, which has never been observed in vivo, possessing both cilia and lamellar bodies was identified in the larger ductular structures. Upon comparison of the ultrastructure of the organoid in vitro cultures in pigskin with the original fetal lung, it was apparent that cytodifferentiation had occurred. The organoid components and structure of the cultured cells more closely resembled adult lung than the fetal lung used to initiate the cultures.

Published

1980

4. Duct, exocrine, and endocrine components of cultured fetal mouse pancreas

Author

Aaron E. Freeman, Koichi Hirata, and Tadashi Oku

Subjects

medicine.medical_specialty, Trypsin inhibitor, Plant Science, Glucagon, Islets of Langerhans, Mice, Internal medicine, medicine, Organoid, Acinar cell, Animals, Amylase, Pancreas, Cells, Cultured, biology, Kunitz STI protease inhibitor, Mesenchymal stem cell, DNA, Hormones, Culture Media, Microscopy, Electron, medicine.anatomical_structure, Endocrinology, Amylases, biology.protein, Cell Division, Biotechnology

Abstract

Twenty to twenty-two days postcoitum mouse fetal pancreas organ bits were cultured on the dermal surface of irradiated pigskin as a substrate. The medium used for long term culture consisted of Eagle’s Minimum Essential Medium with the addition of 10% bovine serum, 0.02 U/ml insulin, 0.025 μg/ml glucagon, 3.63 μg/ml hydrocortisone, 100 μg/ml soybean trypsin inhibitor or 10−8 M atropine. When the medium lacked trypsin inhibitor or atropine but contained the three hormones, the pigskin support began to be destroyed after 2 to 4 wk in culture. Thereafter, the cultured cells could not grow and survive on the digested pigskin. When 10−6 M atropine was added to the medium, amylase secretion from cultured cells and destruction of pigskin were inhibited completely but pancreas cells could not grow or survive. In contrast, 100 μg/ml soybean trypsin inhibitor or 10−8 M atropine permitted cell growth, permitted amylase secretion from the cultured acinar cells, and prevented the destruction of pigskin. Under these conditions pancreas cells migrated or grew or both from the organ bits onto the surface of the pigskin dermis and organoid aggregations formed. Hydrocortisone was needed to permit growth for more than 2 wk. Glucagon and insulin had additive effects. Light and electron microscopic observations indicated the culture of at least five kinds of cells, i.e., duct, acinar, centroacinar, endocrine, and mesenchymal. The majority of cultured cells were duct cells and acinar cells. There were few mesenchymal cells. Mouse pancreas cells were cultured for at least 12 wk by this method.

Published

1982

5. [Untitled]

Author

Yutaka YOSHIDA, Takashi TOMOYORI, Michio MORI, Koichi HIRATA, and Aaron E. FREEMAN

Subjects

Hepatology

Published

1983

6. Problems in Interpretation of Experimental Evidence of Cell Transformation

Author

Robert J. Huebner and Aaron E. Freeman

Subjects

Cancer Research, Cell-Free System, DNA Viruses, Biology, Transformation (music), Adenoviridae, Cell Line, Interpretation (model theory), Theoretical physics, Cell Transformation, Neoplastic, Oncology, RNA Viruses, Oncogenic Viruses, Antigens, Viral

Published

1973

7. 5-Bromo-2′-deoxyuridine Potentiation of Transformation of Rat-Embryo Cells Induced In Vitro by 3-Methylcholanthrene: Induction of Rat Leukemia Virus gs Antigen in Transformed Cells

Author

Robert J. Huebner, Patricia E. Hugunin, Aaron E. Freeman, Mina Lee Vernon, Raymond V. Gilden, and Ronald G. Wolford

Subjects

Immunodiffusion, Cell, Virus Replication, Virus, Cell Line, chemistry.chemical_compound, Antigen, medicine, Animals, Antigens, Viral, Multidisciplinary, biology, Complement Fixation Tests, Drug Synergism, RNA-Directed DNA Polymerase, RNA virus, Embryo, Mammalian, biology.organism_classification, Molecular biology, Deoxyuridine, Rats, Microscopy, Electron, Cell Transformation, Neoplastic, Retroviridae, medicine.anatomical_structure, Bromodeoxyuridine, chemistry, Cell culture, Methylcholanthrene, Biological Sciences: Immunology

Abstract

Low-passage rat-embryo cells were not transformed by 3-methylcholanthrene or by 5-bromo-2′ deoxyuridine. However, prior treatment with bromodeoxyuridine, followed by treatment with methylcholanthrene, resulted in cell transformation about three subpassages after removal of the carcinogen. RNA-directed DNA polymerase activity could not be detected in either normal or transformed cells. However, gs-1 antigen specific for rat C-type RNA virus was detected in cultures derived from bromodeoxyuridine-treated cells. No gs-1 antigen for the C-type RNA virus was detected in cultures that had not been treated with bromodeoxyuridine during the 25 subpassages of these experiments. High-passage rat-embryo cells, derived from a different cell pool, were transformed by either methylcholanthrene or dimethylbenzanthracene without prior infection with an exogenous virus, and without prior treatment with bromodeoxyuridine, gs-1 antigen for C-type RNA virus was also detected in 4 of 4 randomly selected transformed cell lines; the gs-1 antigen was not detected in any of 4 nontransformed control cultures. Considering these and previously published findings, we conclude that the lowpassage cells cannot be transformed by methylcholanthrene because of powerful cellular controls over the endogenous virus. Bromodeoxyuridine triggers some expressions of the endogenous virus; thus, the bromodeoxyuridine-treated cells are more susceptible to the transforming effects of methylcholanthrene. High-passage rat cells do not maintain perfect control over expression of their endogenous virus; the cell cultures are susceptible to the transforming effects of chemical carcinogens.

Published

1973

8. A simple interferon assay as an adjunct for determining the genus of origin of cell cultures

Author

Aaron E. Freeman, Paul J. Price, Zenobia Holbrook, Carol P. Uhlendorf, and Eugene M. Zimmerman

Subjects

Sindbis virus, Cell type, Fibrosarcoma, Cytological Techniques, Newcastle disease virus, Mice, Inbred Strains, Plant Science, Kidney, Vesicular stomatitis Indiana virus, Cell Line, Mice, Cytopathogenic Effect, Viral, Species Specificity, Interferon, Rats, Inbred BN, biology.animal, medicine, Animals, Humans, Primate, Skin, biology, Muscles, Haplorhini, Fibroblasts, Orthomyxoviridae, biology.organism_classification, Virology, In vitro, Rats, Vesicular stomatitis virus, Cell culture, Karyotyping, Interferons, Rabbits, Sindbis Virus, African Green Monkey, Biotechnology, medicine.drug

Abstract

A short, simple test involving interferon-mediated protection of cells in vitro from cytopathogenic effects produced by vesicular stomatitis virus or Sindbis virus has been developed to help in determining the genus of origin of cells. By using the observed pattern of protection of five cell types by five interferons, cells could be grouped as of primate, rabbit, rat, and mouse origins. The primate grouping resulted from bilateral cross-reactions between the human and monkey systems. An unexpected observation was that African green monkey interferon preparations protect both monkey and rat cells, but not the converse. Chromosomal analysis of the cell cultures confirmed the genus determined by the interferon test.

Published

1972

9. THE AMINO ACID REQUIREMENTS OF MONKEY KIDNEY CELLS IN FIRST CULTURE PASSAGE

Author

Harry Eagle, Mina. Levy, and Aaron E. Freeman

Subjects

chemistry.chemical_classification, Arginine, Glutamine, Immunology, Glutamic acid, Haplorhini, Biology, Kidney, Molecular biology, Article, Amino acid, Cell Line, chemistry, Biochemistry, Cell culture, Immunology and Allergy, Animals, Tyrosine, Asparagine, Subculture (biology), Amino Acids, Amino acid synthesis

Abstract

Monkey kidney cells tested in their first culture passage, 24 hours after their isolation from the animal host, required the same 13 amino acids for survival and growth as cell lines serially propagated in culture for years. Under the conditions of the present experiments, arginine, cystine, glutamine, histidine, and tyrosine proved necessary, over and above the 8 amino acids required for nitrogen balance in man. With the serially propagated lines, glutamic acid substituted for glutamine only at extremely high and non-physiological levels. In the monkey kidney cell cultures, however, glutamic acid and glutamine were interchangeable, mole for mole; and aspartic acid and asparagine were also effective as glutamine substitutes. Glycine was growth-stimulatory for monkey kidney cells in primary culture, and the cells grown in a glycine-deficient medium usually failed to survive subculture.

Published

1958

10. Characterisation of human cells transformed in vitro by urethane

Author

Howard J. Igel, Peter A. Jones, Walter E. Laug, William F. Benedict, and Aaron E. Freeman

Subjects

education.field_of_study, Multidisciplinary, Fibrinolysis, Population, Osteitis Fibrosa Cystica, Familial disorder, Biology, Aneuploidy, Urethane, Molecular biology, In vitro, Cell Line, Malignant transformation, Transformation (genetics), Cell Transformation, Neoplastic, Cell culture, Karyotyping, Humans, Animal species, education, Gene

Abstract

CELLS derived from several animal species, including mouse1,2, hamster3 and rat4, have been transformed in vitro from the normal to the malignant state by diverse chemical carcinogens. In similar conditions, however, attempts to transform human cells have usually been unsuccessful and as far as we know, such transformation has been reported only once5. This was a case of two cell lines treated with urethane, obtained from siblings with von Recklinghausen's disease, a familial disorder transmitted by an autosomal dominant gene, and characterised by multiple fibromas with a high predisposition to malignant transformation in vivo6. Although morphologically altered foci of transformed cells were reported, there was the possibility that a few tumour cells in the original population had been selected for by urethane. Therefore we characterised in detail the urethane-treated and untreated cultures. We have found that human cells can indeed be chemically transformed in vitro.

Published

1975

11. Prevention of viral-chemical co-carcinogenesis in vitro by type-specific anti-viral antibody

Author

Aaron E. Freeman, Martin P. King, Raymond V. Gilden, Robert J. Huebner, Teresa M. Bellew, and Paul J. Price

Subjects

Multidisciplinary, biology, viruses, Viral transformation, biology.organism_classification, medicine.disease, Antibodies, Viral, Virology, Molecular biology, Rauscher Virus, Virus, Cell Line, chemistry.chemical_compound, Leukemia, Cell Transformation, Neoplastic, chemistry, Cell culture, Murine leukemia virus, Methylcholanthrene, biology.protein, medicine, Radiation Leukemia Virus, Neutralizing antibody, Research Article

Abstract

Low passage Fischer rat embryo cultures, which are normally very resistant to transformation by 3-methylcholanthrene but are highly susceptible when chronically infected with the Rauscher murine leukemia virus, were completely protected from transformation by methylcholanthrene when treated with neutralizing antibody specific for the leukemia virus prior to and during treatment with methylcholanthrene. Sister cultures were not protected by neutralizing antibody specific for the B-tropic radiation leukemia virus. This demonstrates clearly a definite type specific role for Rauscher murine leukemia virus in the 2-methylcholanthrene transformation system in rat cells.

Published

1976

12. Modulation of fetal mouse liver cells cultured on a pigskin substrate

Author

Koji Shiramatsu, Hiroshi Hayasaka, Koichi Hirata, Tomoaki Usui, Yutaka Yoshida, and Aaron E. Freeman

Subjects

Hydrocortisone, Swine, Biology, General Biochemistry, Genetics and Molecular Biology, Mice, Fetus, Pregnancy, Albumins, Parenchyma, medicine, Transferase, Animals, Cells, Cultured, chemistry.chemical_classification, Basement membrane, L-Lactate Dehydrogenase, Albumin, Esterases, Substrate (chemistry), Cell Differentiation, General Medicine, DNA, gamma-Glutamyltransferase, Molecular biology, digestive system diseases, Culture Media, Enzyme, medicine.anatomical_structure, chemistry, Biochemistry, Liver, Female, alpha-Fetoproteins, Epidermis, medicine.drug

Abstract

HIRATA, K., SHIRAMATSU, K., USUI, T., YOSHIDA, Y., FREEMAN, A.E. and HAYASAKA, H. Modulation of Fetal Mouse Liver Cells Cultured on a Pigskin Substrate. Tohoku J. exp. Med., 1983, 140, (1), 15-28-Mouse fetal liver cells cultured on a pigskin epidermal substrate grew for 7 weeks. Different enzymes and proteins, i.e. gamma-glutamyl transferase (GGT), nonspecific esterase (NE), lactic dehydrogenase (LDH), alpha-fetoprotein (AFP), and albumin were studied histochemically and/or biochemically. The activity of GGT was high at the beginning of culture and then decreased rapidly. The activities of NE and LDH were high during the culture. Release into the media and localization of AFP suggested active synthesis during the early stages. AFP levels gradually decreased and could be demonstrated only in trace amounts after 3-4 weeks of culture. On the other hand, the production of albumin was weakly evident early and became more and more evident after the second week in culture. Hydrocortisone modulated AFP and albumin production. The effect of hydrocortisone was to prolong expression of AFP and to reduce expression of albumin. Electron microscopic observations showed that the cultures consisted of organelle-rich parenchymal cells associated with the pigskin basement membrane by pseudopod-like structures. These results indicate that fetal mouse parenchymal cells were cultured and modulated on a pigskin epidermal substrate.

Published

1983

13. Heteroploid conversion of human skin cells by methylcholanthrene

Author

Howard J. Igel, Lisa Gernand, James M. Malone, William F. Benedict, Mary Rose Pezzutti, Robert S. Lake, Aaron E. Freeman, and Corey Mark

Subjects

Male, Adolescent, Population, Cell, Aneuploidy, Human skin, Biology, Chromosomes, Epithelium, chemistry.chemical_compound, Skin Physiological Phenomena, medicine, Humans, education, Child, Carcinogen, Cells, Cultured, Skin, education.field_of_study, Multidisciplinary, Infant, Newborn, Infant, Fibroblasts, medicine.disease, Molecular biology, medicine.anatomical_structure, chemistry, Bromodeoxyuridine, Immunology, Methylcholanthrene, Female, Research Article

Abstract

Cultured epithelial cells from human skin generally had 3- to 30-fold more hydrocarbon-metabolizing activity than fibroblasts from skin of the same donor. This activity was constant for up to 55 days in primary culture but was lost rapidly upon physical subdivision of the cultures. Treatment of primary mixed fibroblasts and epithelial cell cultures with methylcholanthrene, but not phenanthrene, led to development of actively growing fibroblastic cultures with many heteroploid cells. Unique marker chromosomes, stable over a number of cell population doublings, were identified in several of the heteroploid cell strains. Pure cultures of fibroblasts from the same donors did not undergo heteroploid conversion in response to methylcholanthrene. Spontaneously occurring heteroploidy in logarithmic phase human fibroblasts is a rare event; thus, heteroploid conversion may be a useful marker for chemical transformation of human cells. Because methylcholanthrene seems to have little transforming effect on human skin fibroblasts, human skin epithelial cells, because of their hydrocarbon-metabolizing activity, may serve to convert methylcholanthrene from a distal to an ultimate carcinogenic form.

Published

1977

14. Laminin and fibronectin in cell adhesion: enhanced adhesion of cells from regenerating liver to laminin

Author

Aaron E. Freeman, Roland N.K. Carlsson, Eva Engvall, and Erkki Ruoslahti

Subjects

Basement Membrane, Mice, Laminin, medicine, Cell Adhesion, Animals, Cell adhesion, Egtazic Acid, Glycoproteins, chemistry.chemical_classification, Basement membrane, Multidisciplinary, biology, Regeneration (biology), Membrane Proteins, Fibronectins, Liver regeneration, Cell biology, Liver Regeneration, Fibronectin, medicine.anatomical_structure, chemistry, Biochemistry, Liver, biology.protein, Glycoprotein, Research Article

Abstract

Laminin, a basement membrane glycoprotein isolated from cultures of mouse endodermal cells and rat yolk sac carcinoma cells, promoted the attachment of liver cells obtained from regenerating mouse liver. Cells from normal mouse liver attached readily to dishes coated with fibronectin but attached poorly to surfaces coated with laminin. Both proteins efficiently promoted the attachment of cells from livers undergoing regeneration. After regeneration, the attachment to laminin returned to the low levels found in animals not subjected to partial hepatectomy but attachment to fibronectin remained high. Immunofluorescent staining of sections of normal liver with antilaminin revealed the presence of laminin in or adjacent to the walls of the bile ducts and blood vessels. After induction of regeneration by partial hepatectomy, increased amounts of laminin appeared in the sinusoidal areas. After carbon tetrachloride poisoning, staining for laminin was especially pronounced in the necrotic and postnecrotic areas around the central veins. This additional expression of laminin was transient. It reached a maximum around 5--6 days after the injury and then gradually disappeared. These findings show that laminin is an adhesive protein. The increase of laminin in regenerating liver and the adhesiveness of cells from such livers to laminin suggest a role for laminin in the maintenance of a proper tissue organization during liver regeneration.

Published

1981

15. Differentiation of fetal liver cells in vitro

Author

Koichi Hirata, Virginia Hilborn, Erkki Ruoslahti, Eva Engvall, Yutaka Yoshida, Randall H. Kottel, and Aaron E. Freeman

Subjects

medicine.medical_specialty, Hydrocortisone, Cellular differentiation, Cell, Serum albumin, Mice, Internal medicine, medicine, Animals, Cells, Cultured, Serum Albumin, Embryonic Induction, Fetus, Multidisciplinary, Epidermis (botany), biology, Liver cell, Albumin, Cell Differentiation, In vitro, digestive system diseases, Endocrinology, medicine.anatomical_structure, Liver, embryonic structures, biology.protein, alpha-Fetoproteins, Epidermis, Research Article

Abstract

Fetal mouse liver hepatocytes proliferate on a substrate of irradiated pigskin epidermis scored with scalpel blade slits to permit cell access to the basement membrane. At the time the cells are explanted, fetal genes, such as those responsible for production of alpha-fetoprotein (AFP) and gamma-glutamyltransferase (GGTase), are strongly expressed. The levels of GGTase decrease rapidly and become undetectable within 2 weeks. The levels of AFP decrease more gradually but become undetectable after 3-5 weeks in culture. As the AFP levels decrease, there is a concomitant increase in albumin production. Hydrocortisone prolongs production of AFP (for up to 8 weeks) but not of GGTase, and it decreases albumin production for up to 8 weeks. Once cells lose AFP expression, addition of hydrocortisone does not restart it. Based on these data, fetal mouse liver hepatocytes, cultured on pigskin, seem to be an excellent in vitro model for liver cell maturation.

Published

1981

16. Growth and characterization of human skin epithelial cell cultures

Author

Aaron E. Freeman, Brenda J. Herrman, Karen L. Kleinfeld, and Howard J. Igel

Subjects

A549 cell, Cell growth, Cell, Human skin, Epithelial Cells, Plant Science, Skin Transplantation, Biology, Epithelium, In vitro, Cell biology, Transplantation, medicine.anatomical_structure, Intercellular Junctions, Cell Movement, Karyotyping, medicine, Humans, Transplantation, Homologous, Intracellular, Cell Division, Cells, Cultured, Biotechnology, Skin

Abstract

In 129 of 140 attempts, human skin cells were successfully cultured on the dermal collagen bed of sterile, dead pigskin. Diploid epithelial cells grew selectively on the collagen bed; fibroblasts grew on the glass surfaces of the culture dishes. The cultures could be subdivided physically up to six times at a 1:2 split ratio, but at least 24 to 48 cell generations were produced over the months the cells could be carried. Much of the cell multiplication resulted in maturation into distinct basal, squamous, granular, and keratinized cell layers. The cultured cells were considered epithelial because of their shape, possession of intercellular bridges, desmosomes and tonofibrils, and because they formed maturating epithelium in vitro and upon transplantation back to the original human donor. As the cells grew they digested the pigskin collagen, thus producing clear zones that could be used to monitor and quantitate cell growth. Multiplication of epilthelial cells, rather than migration, was indicated by mitotic figures in colchicine-treated cultures and by DNA synthesis.

Published

1976

17. In vivo-like growth of human tumors in vitro

Author

Robert M. Hoffman and Aaron E. Freeman

Subjects

In Vitro Techniques, Cellular differentiation, Mice, Nude, Biology, Extracellular matrix, Tissue culture, Mice, In vivo, Neoplasms, Biopsy, medicine, Animals, Humans, Cells, Cultured, Multidisciplinary, medicine.diagnostic_test, Cell Differentiation, Neoplasms, Experimental, In vitro, Cell biology, Extracellular Matrix, Immunology, Collagen, Function (biology), Neoplasm Transplantation, Research Article

Abstract

We show that diverse human tumors obtained directly from surgery or biopsy can grow at high frequency in vitro for long periods of time and still maintain many of their in vivo properties. The in vivo properties maintained in vitro include three-dimensional growth; maintenance of tissue organization and structure, including changes associated with oncogenic transformation; retention of differentiated function; tumorigenicity; and the growth of multiple types of cells from a single tumor.

Published

1986

18. Carcinogenesis in vitro. II. Chemical transformation of diploid human cell cultures: A rare event

Author

Karen L. Kleinfeld, Howard J. Igel, Aaron E. Freeman, and Joan E. Spiewak

Subjects

Adult, Neurofibroma, Neurofibromatosis 1, G banding, Contact inhibition, Plant Science, Biology, medicine.disease, medicine.disease_cause, Molecular biology, Diploidy, Urethane, Transformation (genetics), Cell Transformation, Neoplastic, Cell culture, medicine, Humans, Female, Ploidy, Carcinogenesis, Developmental biology, Cells, Cultured, Biotechnology

Abstract

Seventy-five diploid human cell strains were subjected to a number of chemical carcinogens, including urethane and polycyclic hydrocarbons. In most cases, no visible morphological alterations were induced by any treatment. Development of morphologically altered foci was noticed in urethane-treated cultures derived from a patient with von Recklinghausen's disease. This disease is transmitted by an autosomal dominant gene, and has a high rate of spontaneous transformation of neurofibromas to neurofibrosarcomas. Attempts to isolate continuous cell lines from altered foci were successful in only two of several attempts. These continuous cell lines demonstrate altered morphology, loss of contact inhibition, accelerated growth rate, and have attained over 240 generations in a period of 140 weeks. Untreated control cultures became terminal by the 20th generation. Giemsa banding procedures showed that the chromosomal complement consisted of heteroploid human chromosomes. A second diploid cell strain derived from the above patient's sibling, also suffering from von Recklinghausen's disease, likewise was morphologically altered by urethane. Chemical transformation of human cells is difficult to induce; however, selection of genetically predisposed cells and prolonged, intermittent, and repeated chemical treatment may be important factors in achieving transformation.

Published

1975

19. Myo-Inositol as an essential growth factor for normal and malignant human cells in tissue culture

Author

Vance I. Oyama, Aaron E. Freeman, Mina Levy, and Harry Eagle

Subjects

Phytic acid, Multidisciplinary, Growth factor, medicine.medical_treatment, Inositol Metabolism, Cell Biology, Biology, Biochemistry, Tissue Culture Techniques, chemistry.chemical_compound, Tissue culture, chemistry, Cell culture, Research Design, Neoplasms, medicine, Carbohydrate Metabolism, Humans, Intercellular Signaling Peptides and Proteins, Inositol, Molecular Biology

Published

1957

20. Transformation of primary rat embryo cells by adenovirus type 2

Author

Eustace A. Vanderpool, Robert J. Huebner, Aaron E. Freeman, Joan B. Austin, Paul H. Black, and Patrick H. Henry

Subjects

Genetics, Multidisciplinary, Primary (chemistry), Chemistry, Fluorescent Antibody Technique, Embryo, Cell biology, Adenoviridae, Rats, Transformation (genetics), Culture Techniques, Animals, RNA, Calcium, Antigens, Research Article

Published

1967

21. T and tumour antigens of adenovirus group C-infected and transformed cells

Author

Horace C. Turner, Robert C. Mcallister, Robert J. Huebner, Carolyn E. Martin, Jerome Kern, Aaron E. Freeman, and Raymond V. Gilden

Subjects

Human Adenoviruses, Hemagglutination, Cell, Fluorescent Antibody Technique, Biology, Homology (biology), Adenoviridae, Antigen, Cytopathogenic Effect, Viral, Culture Techniques, medicine, Animals, Humans, Antigens, Pan-T antigens, Multidisciplinary, Immune Sera, Complement Fixation Tests, Embryo, Neoplasms, Experimental, Fibroblasts, Embryo, Mammalian, Virology, Molecular biology, Rats, medicine.anatomical_structure, Cell Transformation, Neoplastic, biology.protein, Antibody, Oncogenic Viruses

Abstract

ONCOGENIC human adenoviruses are readily divisible into two chief subgroups: A (types 12, 18, 31), and B (types 3, 7, 14, 16, 21 and probably 11) based on similar biological and biophysical properties1,2. Recently, Freeman et al.3 showed that adenovirus type 2, representative of a third subgroup of human adenoviruses, morphologically transformed rat embryo cells. The viruses of this subgroup, types 1, 2, 5 and 6, are similar in many biologic properties; they produce a partial haemagglutination pattern with rat erythrocytes, the agglutination being enhanced by the presence of heterotypic antibody4. Adenovirus type 4 also partially agglutinates rat cells, but in other respects, such as T antigen reactivity5, DNA–DNA homology6 and homology with tumour cell mRNA7, seems related to the B oncogenic subgroup. The rat cells transformed with adenovirus 2 contain an antigen which reacted in both complement-fixation (CF) and immunofluorescent tests with sera from hamsters inoculated with tumour extracts and with cells transformed by adenovirus 1- and 2-SV40 hybrid viruses3,8. These results suggested, as shown here, that other members of the adenovirus 1, 2, 5 and 6 subgroup would transform rat cells and that a common T antigen could be demonstrated. Evidence obtained by the fluorescent antibody method for a shared T antigen for adenoviruses 1 and 2 has already been reported8.

Published

1968

22. Adenovirus type 12-rat embryo transformation system

Author

Aaron E. Freeman, Robert J. Huebner, Ronald G. Wolford, and Paul H. Black

Subjects

Virus Cultivation, Immunology, chemistry.chemical_element, Calcium, Biology, medicine.disease_cause, Kidney, Microbiology, Adenoviridae, Cell Line, Tissue culture, Cytopathogenic Effect, Viral, Virology, Culture Techniques, Animal Viruses, medicine, Animals, Humans, Mouth neoplasm, Carcinoma, Embryo, Embryo, Mammalian, Molecular biology, Tumor antigen, Transformation (genetics), Cell Transformation, Neoplastic, chemistry, Cell culture, Insect Science, Mouth Neoplasms, Rabbits

Abstract

Adenovirus type 12 (Huie) inoculated into cultures of primary whole rat embryo produced foci of morphologically altered cells. The number and identification of these transformed areas was dependent upon the calcium concentration of the medium; more foci appeared in 0.1 m m than in 1.8 m m calcium. Cell lines derived from these inoculated cultures did not yield infectious virus, and also were similar to cell lines derived from adenovirus type 12-induced tumors with respect to morphology, presence of virus-specific tumor antigen, and oncogenicity. Dose-response curves revealed that transformation of rat embryo cells by adenovirus type 12 followed one-hit kinetics, and that approximately 7 × 10 5 infectious virus particles were required for one transformation event. Our results indicate that the transformation system described for adenovirus type 12 is reproducible, and that previous difficulties experienced in developing such a system may well be explained by the higher calcium concentration of the tissue culture media used.

Published

1967

23. Activation and Isolation of Hamster-Specific C-Type RNA Viruses from Tumors Induced by Cell Cultures Transformed by Chemical Carcinogens

Author

Robert J. Huebner, Aaron E. Freeman, Gary J. Kelloff, Raymond V. Gilden, Ansel P. Swain, and William T. Lane

Subjects

Biological Sciences: Microbiology, Hamster, Tritium, Cell Line, chemistry.chemical_compound, Cricetinae, Smoke, Tobacco, Animals, RNA Viruses, Antigens, Viral, Uridine, Carcinogen, Cells, Cultured, Multidisciplinary, biology, RNA, RNA virus, Embryo, Neoplasms, Experimental, Fibroblasts, biology.organism_classification, Embryo, Mammalian, Virology, Molecular biology, Plants, Toxic, Cell Transformation, Neoplastic, chemistry, Cell culture, Methylcholanthrene, Carcinogens, Autoradiography, RNA, Viral

Abstract

Cell cultures of Syrian hamster embryo were treated for 7 days with selected chemicals. Certain cultures were morphologically transformed by three different chemical preparations and yielded cell lines that subsequently produced malignant tumors in hamsters. Although the cell lines were negative for infectious virus before inoculation into animals, hamster-specific C-type RNA virus was isolated from tumors or from cell lines derived from the tumors. Since infectious C-type viruses are usually not demonstrable in hamster tissues of normal or tumor origin, we conclude that the chemical treatment and activation of the viruses are related events.

Published

1971

24. Type C RNA Tumor Viruses as Determinants of Chemical Carcinogenesis: Effects of Sequence of Treatment

Author

William A. Suk, Aaron E. Freeman, and Paul J. Price

Subjects

Time Factors, Multidisciplinary, viruses, RNA, Embryo, Viral transformation, Biology, Embryo, Mammalian, medicine.disease_cause, biology.organism_classification, Rauscher Virus, Virology, Molecular biology, Virus, Cell Line, Rats, Transformation (genetics), Cell Transformation, Neoplastic, Murine leukemia virus, Tumor Virus, medicine, Animals, Carcinogenesis, Cells, Cultured, Methylcholanthrene

Abstract

Fischer rat embryo cells were treated with 3-methylcholanthrene before or after inoculation with Rauscher murine leukemia virus. Transformation was not observed in untreated control cultures, cultures given virus or 3-methyl-cholanthrene alone, or cultures treated first with 3-methylcholanthrene followed by inoculation with the virus after removal of the chemical. Transformation was dependent upon the presence of Rauscher murine leukemia virus at the time of chemical treatment.

Published

1972

25. International Cooperation in Radiobiology through an Agency Sponsored by the United Nations

Author

Aaron E. Freeman, Mina Levy, Harry Eagle, and Vance I. Oyama

Subjects

medicine.medical_specialty, chemistry.chemical_compound, Tissue culture, Multidisciplinary, Endocrinology, chemistry, Internal medicine, Growth factor, medicine.medical_treatment, medicine, Cancer research, Inositol

Published

1956