AI Article Synopsis
- Researchers studied how normal human mammary epithelial cells (HME87) respond to the carcinogen benzo[a]pyrene diol epoxide (BPDE), finding that after 24 hours of treatment, the cells didn’t undergo typical cell cycle arrest or apoptosis despite a 50% reduction in cell number.
- Gene expression analysis using the RAGE technique revealed that while some genes related to DNA damage response were activated early, the p21-WAF1 gene, which prevents cells from moving from G(1) to S phase, only increased after 24 hours.
- The study highlighted significant changes in gene expression, including transcription factors like ATF3 and E2A, and noted that BPDE treatment led to early
Article Abstract
The responses of a line of normal human mammary epithelial cells, HME87, to treatment with the ultimate carcinogen benzo[a]pyrene diol epoxide (BPDE) were analyzed using a directed gene expression analysis technique, RAGE. Under conditions where cell number was decreased by 50% 24 or 48 h post-treatment, flow cytometry demonstrated no establishment of a G(1)/S arrest nor induction of apoptosis; cells continued to enter S phase from G(1) for at least 24 h but were blocked at G(2)/M. Using the RAGE technique, changes in gene expression were assayed for over 1000 genes, and multiple time-point data were collected for approximately 90 genes. In accord with the cell cycle studies, expression of the p21-WAF1 gene, the major mediator of p53-dependent G(1)/S arrest, did not increase until 24 h post-treatment. The expression of other target genes for transactivation by p53 was increased at early time points, including GADD45, an effector of the G(2)/M checkpoint, and WIP1. Analyses of proteins in treated cells indicated that p53 was phosphorylated at Ser15 but not at Ser20 within 30 min of treatment, and this correlated with an increase in the total amount of p53 protein. Significant expression changes were noted in a number of transcription factor genes, including ATF3 and E2A, genes that have not been previously connected to a response to DNA damage involving bulky chemical adducts. In addition, expression of the XPC gene was induced by BPDE treatment; the XPC product is thought to be involved in recognition of DNA damage by the nucleotide excision repair system.
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| http://dx.doi.org/10.1093/carcin/24.2.225 | DOI Listing |
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