Increase in wild-type p53 stability and transactivational activity by the chemopreventive agent apigenin in keratinocytes

doi:10.1093/carcin/21.4.633

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Carcinogenesis, Vol. 21, No. 4, 633-639, April 2000
© 2000 Oxford University Press

Molecular Epidemiology and Cancer Prevention

Increase in wild-type p53 stability and transactivational activity by the chemopreventive agent apigenin in keratinocytes

Maralee McVean¹, Hengyi Xiao³, Ken-ichi Isobe³ and Jill C. Pelling¹^,2^,4

¹ Department of Pathology and Laboratory Medicine and
² Department of Biochemistry and Molecular Biology, University of Kansas Medical Center, Kansas City, KS 66160, USA and
³ Department of Basic Gerontology National Institute for Longevity Sciences, 36-3 Gengo Morioka-Cho Obu, Aichi 474-8522, Japan

Apigenin, a naturally occurring, non-mutagenic flavonoid, hasbeen shown to inhibit UV-induced skin tumorigenesis in micewhen topically applied. In this report we have used the mousekeratinocyte 308 cell line, which contains a wild-type p53 gene,to study the effect of apigenin treatment on p53 protein levelsand the expression of its downstream partner, p21/waf1. Cellswere treated with 70 µM apigenin for various times andlevels of p53 and p21/waf1 protein were assessed by westernblot analysis. The level of p53 protein was induced 27-foldafter 4 h of apigenin treatment and levels remained elevatedthrough 10 h of exposure. After 24 h of exposure to 70 µMapigenin, p53 protein levels returned to control levels. p21/waf1protein levels increased ~1.5–2-fold after 4 h and remainedelevated at 24 h. To investigate the mechanism of p53 proteinaccumulation, we compared the half-life of p53 protein in vehicle-and apigenin-treated cells. Cells were incubated for 4 h inthe presence of apigenin, then cycloheximide was added to inhibitfurther protein synthesis and p53 protein levels were measuredby western blot. The half-life of p53 protein was found to beincreased an average of 8-fold in apigenin-treated cells comparedwith vehicle-treated cells (t $1/2$ = 131 min versus 16 min in apigenin-versus vehicle-treated cells, respectively). The mechanism ofp53 protein stabilization is currently being investigated. Todetermine whether p53 was transcriptionally active, we alsoperformed gel mobility shift assays and transient transfectionstudies using a luciferase plasmid under the control of thep21/waf1 promoter. Both p53 DNA-binding activity and transcriptionalactivation peaked after 24 h of exposure to apigenin. Thesestudies suggest that apigenin may exert anti-tumorigenic activityby stimulating the p53–p21/waf1 response pathway.

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