Development and characteristics of a human cell assay for screening agents for melanoma prevention

Development and characteristics of a human cell assay for screening agents for melanoma prevention

This paper describes the development and initial evaluation of a human cell assay to identify potentially efficacious agents for preventing melanoma. Four human cell lines were used: normal melanocytes, a radial growth-phase-like melanoma cell line (WM3211), a vertical growth-phase-like melanoma cel...

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Veröffentlicht in:Melanoma research 2007-02, Vol.17 (1), p.42-50
Hauptverfasser: Elmore, Eugene, Jain, Aarti, Siddiqui, Shazia, Tohidian, Nilou, Meyskens, Frank L, Steele, Vernon E, Redpath, John L
Format: Artikel
Sprache:eng
Schlagworte:
Annexin A5 - analysis
Cadherins - analysis
Cell Line
Cell Line, Tumor
Foreskin - cytology
Humans
Infant, Newborn
Male
Mass Screening - methods
Melanocytes - cytology
Melanocytes - pathology
Melanoma - epidemiology
Melanoma - prevention & control
Reproducibility of Results
Skin Neoplasms - epidemiology
Skin Neoplasms - prevention & control
Ultraviolet Rays
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Zusammenfassung:This paper describes the development and initial evaluation of a human cell assay to identify potentially efficacious agents for preventing melanoma. Four human cell lines were used: normal melanocytes, a radial growth-phase-like melanoma cell line (WM3211), a vertical growth-phase-like melanoma cell line (Lu1205), and 83-2c, a cell strain cloned from metastatic melanoma. Four endpoints were evaluated in ultraviolet B-treated cells: annexin V, human leukocyte antigen-DR; E-cadherin, and N-cadherin. Annexin V was induced by nimesulide, 4-hydroxyphenylretinamide, and difluoromethylornithine in ultraviolet-B-treated radial growth-phase-like melanoma cells. None of the agents inhibited human leukocyte antigen-DR expression in ultraviolet-B-treated radial growth-phase-like melanoma cells, the only cells that strongly expressed human leukocyte antigen-DR. E-cadherin was overexpressed only in radial growth-phase-like melanoma cells relative to melanocytes, and ultraviolet B exposure dramatically reduced this expression. E-cadherin was only induced by difluoromethylornithine in ultraviolet-B-treated radial growth-phase-like melanoma cells. N-cadherin was over- expressed in all melanoma cell lines relative to melanocytes. In this study, all candidate preventive agents inhibited N-cadherin in ultraviolet B-treated radial growth-phase-like melanoma cells. Four agents inhibited N-cadherin in ultraviolet B-treated vertical growth-phase-like melanoma cells. The mean ratios of N-cadherin to E-cadherin levels and specific endpoint responses for both the radial growth-phase-like melanoma and vertical growth-phase-like melanoma cells were used to rank the agents. Agents were evaluated at clinically relevant concentrations. The rankings were difluoromethylornithine>4-hydroxyphenylretinamide>nimesulide>9-cis-retinoic acid>polyphenon E. Diphenylhydramine, D-mannitol, and nordihydroguaiaretic acid were inactive. The results of these initial studies suggest that ultraviolet-B-treated radial growth-phase-like melanoma cells are the most responsive to chemopreventive agents, and may be the cell line of choice for screening melanoma prevention agents.
ISSN:0960-8931
DOI:10.1097/cmr.0b013e3280142f96