Human Neoplastic and Normal Cells in Tissue Culture. I. Cell Lines Derived From Malignant Melanomas and Normal Melanocytes2

Bc, Glovanella; Js, Stehlin; Santamaria, Carolina; So, Yim; Ac, Morgan; Lj, Williams; Leibovitz, Albert; Pj, Fialkow; Dm, Mumford

doi:10.1093/jnci/56.6.1131

Cited by 68 publications

(16 citation statements)

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“…The two cell lines in this series that did pigment in culture were similar to those described by Romsdahl and Hsu (1972) and Giovanella et al (1976) in that melanogenesis increased with increasing cell density. In our experience cell clusters that formed at confluence were particularly deeply pigmented.…”

Section: Resultssupporting

confidence: 83%

Characterization of seven human melanoma cell lines: Melanogenesis and secretion of plasminogen activators

Helden¹,

Wilson²,

Dowdle³

1986

Br J Cancer

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Summary Permanent cell lines (UCT-Mel 1 through 7) were established from biopsies of metastatic tissue taken from seven patients with malignant melanoma. Cells from these lines were all aneuploid and all grew as non-contact-inhibited, adherent monolayers. All of the lines, with the remarkable exception of UCT-Mel 6, formed tumours in nude mice, expressed the melanoma M-18 antigen and synthesized plasminogen activators exclusively of the tissue-type. UCT-Mel 6 cells were non tumourigenic, they lacked the M-18 antigen and they synthesized plasminogen activators exclusively of the urokinase type. UCT-Mel I and UCT-Mel 2 formed pigment in vitro and both of these lines showed an increase in pigment content and tyrosinase synthesis with increasing cell density. The rate of plasminogen activator released by UCT-Mel 1 and UCT-Mel 3 declined strikingly as the cells became confluent.Assuming (a) that proteolytic activity is required for cell migration in vivo; (b) that tyrosinase synthesis reflects expression of the differentiated phenotype and (c) that melanoma cells retain some of the characteristics of neural crest cells, we suggest that the effects of confluence and close cell-cell contact provide a useful experimental counterpart for the study of normal neural crest all behaviour that is characterized by an inverse relationship between migration and a protease secretion on the one hand and pigmentation on the other.Human melanoma cells cultured in vitro provide a useful system for examining processes that are relevant both to this particular class of tumours and, at the same time, to cellular biological phenomena of a more general nature.Melanogenesis, for example, is an obvious and readily quantifiable marker of cellular differentiation that can be used to study factors that govern expression of the differentiated phenotype in pigmenting cell lines. Furthermore, as derivatives of the embryonic neural crest, melanoma cells share a common origin with a variety of ectomesenchymal structures, cells of the autonomic nervous system, calcitonin-producing cells, cells of the carotid body and sensory neurones in spinal ganglia and cranial nerves. It is now clear that, in choosing one of these diverse alternative destinies, pluripotential neural crest 'stem-cells' are influenced by environmental cues that come from neighbouring embryonic structures (Le Douarin, 1982 serum (State Vaccine Laboratories, Cape Town), 300 g penicillin ml-1, 200, g streptomycin sulphate ml-1 and 10 yg tylocine ml-1. Cultures were maintained at 37°C in a humid atmosphere containing 5% CO2 in air.Culture media were changed twice weekly. Confluent adherent cultures were passaged by detachment with 0.25% trypsin and 0.02% EDTA in Tris-buffered saline (TBS: 0.137 M NaCl, 5 mM KCl, 0.7 mM Na Phosphate, 25 mM TrisHCl; pH7.4) and re-seeding at -2x 105 cells/ 35 mm dish.Cell lines were tested for mycoplasma contamination (Chen, 1977) and found to be negative.Growth curves were constructed by seeding cells at a low density (usually 105 cells/35mm dish) and fe...

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Section: Resultssupporting

confidence: 83%

Characterization of seven human melanoma cell lines: Melanogenesis and secretion of plasminogen activators

Helden¹,

Wilson²,

Dowdle³

1986

Br J Cancer

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“…HO-1 and MeWo are established human melanotic melanoma cell lines and FO-1 is an established human amelanotic melanoma cell line isolated from separate patient-derived metastatic lesions (Giovanella et al, 1976;Kerbel et al, 1994;Fisher et al, 1985;Graham et al, 1991). WM35 was derived from an RGP primary human melanoma (Herlyn, 1990).…”

Section: Cell Lines and Culture Conditionsmentioning

confidence: 99%

The cancer growth suppressing gene mda-7 induces apoptosis selectively in human melanoma cells

et al. 2002

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Human melanoma cells growth arrest irreversibly, lose tumorigenic potential and terminally di erentiate after treatment with a combination of ®broblast interferon (IFN-b) and the protein kinase C activator mezerein (MEZ). Applying subtraction hybridization to this model di erentiation system permitted cloning of melanoma di erentiation associated gene-7, mda-7. Expression of mda-7 inversely correlates with melanoma development and progression, with elevated expression in normal melanocytes and nevi and increasingly reduced expression in radial growth phase, vertical growth phase and metastatic melanoma. When expressed by means of a replication incompetent adenovirus (Ad.mda-7) growth of melanoma, but not normal early passage or immortal human melanocytes, is dramatically suppressed and cells undergo programmed cell death (apoptosis). Infection of metastatic melanoma cells with Ad.mda-7 results in an increase in cells in the G 2 /M phase of the cell cycle and changes in the ratio of pro-apoptotic (BAX, BAK) to anti-apoptotic (BCL-2, BCL-XL) proteins. Ad.mda-7 infection results in a temporal increase in mda-7 mRNA and intracellular MDA-7 protein in most of the melanocyte/melanoma cell lines and secretion of MDA-7 protein is readily detected following Ad.mda-7 infection of both melanocytes and melanoma cells. The present studies document a di erential response of melanocytes versus melanoma cells to ectopic expression of mda-7 and support future applications of mda-7 for the genebased therapy of metastatic melanoma.

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“…The HO-1 human melanoma cell line was established from a metastatic inguinal lymph node lesion from a 49 year-old female (Giovanella et al, 1976;. HeLa is a human cervical carcinoma cell line (Kao and Nevins, 1983).…”

Section: Cell Lines and Culture Conditionsmentioning

confidence: 99%

Suppression of human ribosomal protein L23A expression during cell growth inhibition by interferon-β

et al. 1997

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Interferons inhibit cell growth in normal and tumorderived cells. The molecular basis of interferons antiproliferative activity remains to be de®ned. Using subtraction hybridization, a human melanoma dierentiation associated gene, mda-20, has been identi®ed that is down-regulated by treatment with interferon. Sequence analysis indicates that mda-20 is human ribosomal protein L23a (rp L23a). The mRNA levels of rp L23a and growth are diminished in a variety of human tumor cell lines following treatment with human ®broblast interferon, interferon-b (IFN-b). Expression of rp L23a is also reduced in human melanoma cells treated with human leukocyte (IFN-a) and immune (IFN-g) interferons, but not by growth inhibition resulting from serum starvation. These ®ndings suggest that growth suppression alone is not sucient to reduce rp L23a expression. Instead, reduced rp L23a mRNA results from biochemical changes mediated by interferons. Ectopic expression of an antisense rp L23a sequence in human HeLa cervical carcinoma cells results in a reduction in colony formation indicating a direct antiproliferative eect by inhibiting rp L23a expression. The mechanism underlying inhibition in rp L23a expression in IFN-b-treated cells may involve antisense rp L23a RNA. These results suggest that rp L23a may be one of the target molecules involved in mediating growth inhibition by interferon.

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Human Neoplastic and Normal Cells in Tissue Culture. I. Cell Lines Derived From Malignant Melanomas and Normal Melanocytes2

Cited by 68 publications

References 0 publications

Characterization of seven human melanoma cell lines: Melanogenesis and secretion of plasminogen activators

Characterization of seven human melanoma cell lines: Melanogenesis and secretion of plasminogen activators

The cancer growth suppressing gene mda-7 induces apoptosis selectively in human melanoma cells

Suppression of human ribosomal protein L23A expression during cell growth inhibition by interferon-β

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