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Enhancement of melanotic expression in cultured mouse smelanoma cells by retinoids
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AbstractRetinoic acid (RA), which reduces the rate of cell proliferation in S91 mouse melanoma clone C2 cells, was found to stimulate the expression of their melanotic phenotype. RA treatment also induced the extension of long cellular processes. The RA effects on melanogenesis included stimulation of tyrosinase activity and augmentation of cellular melanin content to levels 3‐ to 4‐fold higher than in untreated cultures at similar cell densities. These effects became apparent after 48 hours of exposure to 10−5 M RA and increased thereafter. Halfmaximal stimulation in cells treated for 6 days occurred at 5 × 10−7 M RA. Although the degrees of melanogenesis enhancement by RA (10−5 M) and by α‐melanocyte stimulatory hormone (2 × 10−7 M) were similar, the former did not alter the intracellular cAMP level, whereas the latter induced a transient 4‐fold increase. In high‐passage (p28) cells, as well as in low‐passage cells (< p10) treated with tyrosinase inhibitor phenylthiocarbamate, melanin synthesis was suppressed in the absence and presence of RA, yet the ability of RA to inhibit cell proliferation was not compromised. In the presence of the tumor promotor phorbol myristate acetate (> 5 × 10−9 M) melanin synthesis in control as well as in cells exposed to RA was dramatically inhibited. Phorbol which is not active in tumor promotion had no effect on melanogenesis. In addition to RA, other retinoids, such as 13‐cis‐retinoic acid, retinyl acetate, the TMMP analog of RA and the phenyl analog of RA, but not the pyridyl analog of RA or retinyl palmitate, also inhibited cell growth and enhanced melanin synthesis.
Title: Enhancement of melanotic expression in cultured mouse smelanoma cells by retinoids
Description:
AbstractRetinoic acid (RA), which reduces the rate of cell proliferation in S91 mouse melanoma clone C2 cells, was found to stimulate the expression of their melanotic phenotype.
RA treatment also induced the extension of long cellular processes.
The RA effects on melanogenesis included stimulation of tyrosinase activity and augmentation of cellular melanin content to levels 3‐ to 4‐fold higher than in untreated cultures at similar cell densities.
These effects became apparent after 48 hours of exposure to 10−5 M RA and increased thereafter.
Halfmaximal stimulation in cells treated for 6 days occurred at 5 × 10−7 M RA.
Although the degrees of melanogenesis enhancement by RA (10−5 M) and by α‐melanocyte stimulatory hormone (2 × 10−7 M) were similar, the former did not alter the intracellular cAMP level, whereas the latter induced a transient 4‐fold increase.
In high‐passage (p28) cells, as well as in low‐passage cells (< p10) treated with tyrosinase inhibitor phenylthiocarbamate, melanin synthesis was suppressed in the absence and presence of RA, yet the ability of RA to inhibit cell proliferation was not compromised.
In the presence of the tumor promotor phorbol myristate acetate (> 5 × 10−9 M) melanin synthesis in control as well as in cells exposed to RA was dramatically inhibited.
Phorbol which is not active in tumor promotion had no effect on melanogenesis.
In addition to RA, other retinoids, such as 13‐cis‐retinoic acid, retinyl acetate, the TMMP analog of RA and the phenyl analog of RA, but not the pyridyl analog of RA or retinyl palmitate, also inhibited cell growth and enhanced melanin synthesis.
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