Ultraviolet radiation is the main cause of skin cancers, and melanoma is the most serious form of tumor. There is no therapy for advanced-stage melanoma and its metastasis because of their high resistance to various anticancer therapies. Human skin is an important metabolic organ in which occurs photoinduced synthesis of vitamin D3 from7-dehydrocholesterol (7-DHC). 7-DHC, the precursor of cholesterol biosynthesis, is highly reactive and easily modifiable to produce 7-DHC-derived compounds. The intracellular levels of 7-DHC or its derivatives can have deleterious effects on cellular functionality and viability.In this study we evaluated the effects on melanoma cell lines of 7-DHC as such and for this aim we used much care to minimize 7-DHC modifications. We found that from 12 to 72 h of treatment 82–86% of 7-DHC entered the cells, and the levels of 7-DHC-derived compounds were not significant. Simultaneously, reactive oxygen species production was significantly increased already after 2 h. After 24 h and up to 72 h, 7-DHC-treated melanoma cells showed a reduction in cell growth and viability. The cytotoxic effect of 7-DHC was associated with an increase in Bax levels, decrease in Bcl-2/Bax ratio, reduction of mitochondrial membrane potential, increase in apoptosis-inducing factor levels, unchanged caspase-3 activity, and absence of cleavage of PARP-1. These findings could explain the mechanism through which 7-DHC exerts its cytotoxic effects. This is the first report in which the biological effects found in melanoma cells are mainly attributable to 7-DHC as such.

Evaluation of cytotoxic effects of 7-dehydrocholesterol on melanoma cells / Gelzo, Monica; Granato, Giuseppina; Albano, Francesco; Arcucci, Alessandro; DELLO RUSSO, Antonio; DE VENDITTIS, Emmanuele; Ruocco, MARIA ROSARIA; Corso, G.. - In: FREE RADICAL BIOLOGY & MEDICINE. - ISSN 0891-5849. - 70:(2014), pp. 129-140. [10.1016/j.freeradbiomed.2014.02.013]

Evaluation of cytotoxic effects of 7-dehydrocholesterol on melanoma cells

GELZO, MONICA;ALBANO, FRANCESCO;ARCUCCI, ALESSANDRO;DELLO RUSSO, ANTONIO;DE VENDITTIS, EMMANUELE;RUOCCO, MARIA ROSARIA
;
2014

Abstract

Ultraviolet radiation is the main cause of skin cancers, and melanoma is the most serious form of tumor. There is no therapy for advanced-stage melanoma and its metastasis because of their high resistance to various anticancer therapies. Human skin is an important metabolic organ in which occurs photoinduced synthesis of vitamin D3 from7-dehydrocholesterol (7-DHC). 7-DHC, the precursor of cholesterol biosynthesis, is highly reactive and easily modifiable to produce 7-DHC-derived compounds. The intracellular levels of 7-DHC or its derivatives can have deleterious effects on cellular functionality and viability.In this study we evaluated the effects on melanoma cell lines of 7-DHC as such and for this aim we used much care to minimize 7-DHC modifications. We found that from 12 to 72 h of treatment 82–86% of 7-DHC entered the cells, and the levels of 7-DHC-derived compounds were not significant. Simultaneously, reactive oxygen species production was significantly increased already after 2 h. After 24 h and up to 72 h, 7-DHC-treated melanoma cells showed a reduction in cell growth and viability. The cytotoxic effect of 7-DHC was associated with an increase in Bax levels, decrease in Bcl-2/Bax ratio, reduction of mitochondrial membrane potential, increase in apoptosis-inducing factor levels, unchanged caspase-3 activity, and absence of cleavage of PARP-1. These findings could explain the mechanism through which 7-DHC exerts its cytotoxic effects. This is the first report in which the biological effects found in melanoma cells are mainly attributable to 7-DHC as such.
2014
Evaluation of cytotoxic effects of 7-dehydrocholesterol on melanoma cells / Gelzo, Monica; Granato, Giuseppina; Albano, Francesco; Arcucci, Alessandro; DELLO RUSSO, Antonio; DE VENDITTIS, Emmanuele; Ruocco, MARIA ROSARIA; Corso, G.. - In: FREE RADICAL BIOLOGY & MEDICINE. - ISSN 0891-5849. - 70:(2014), pp. 129-140. [10.1016/j.freeradbiomed.2014.02.013]
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Utilizza questo identificativo per citare o creare un link a questo documento: https://hdl.handle.net/11588/574001
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