## Silencing of p16 INK4a by methylation of the CpG islands in the promoter region has been found to be an alternative mechanism of inactivation in several tumors. However, in gastric carcinoma, the relationship between methylation status and the transcriptional silencing of the p16 gene remains t
Expression of the p16INK4a gene and methylation pattern of CpG sites in the promoter region in rat tumor cell lines
β Scribed by Kanya Honoki; Toshifumi Tsujiuchi; Toshio Mori; Kazuhiro Yoshitani; Masahiro Tsutsumi; Yoshinori Takakura; Yoshio Mii
- Publisher
- John Wiley and Sons
- Year
- 2003
- Tongue
- English
- Weight
- 112 KB
- Volume
- 39
- Category
- Article
- ISSN
- 0899-1987
- DOI
- 10.1002/mc.10165
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β¦ Synopsis
Abstract
Loss of p16^INK4a^ protein expression has frequently been related to DNA methylation in association with gene silencing. Although the methylation status of exon1Ξ± for p16^INK4a^ involvement in various cancers has been extensively analyzed, it has been pointed out that some inconsistencies existed in its relationship to gene silencing of p16^INK4a^. In this study, we focused on the expression and methylation status in the regions of nt β478 to β201, containing a putative TATA box (nt β401 to β396), and nt β233 to 26, both in a recently cloned 5β² upstream region of rat p16^INK4a^. We showed that rat lung adenocarcinoma RLCNR did not express the p16^INK4a^ gene, whereas rat osteosarcoma COS1NR and malignant fibrous histiocytoma MFH1NR both expressed it at levels similar to normal fibroblasts, even though the region of nt β233 to 26 was hypermethylated in COS1NR rather than RLCNR. In contrast, the CpG islands near the putative TATA box region were consistently methylated in RLCNR, but not in COS1NR and MFH1NR, as well as in normal fibroblasts. Treatment with 5βaza 2β²βdeoxycytidine induced expression of p16^INK4a^ gene in RLCNR after 48 h, but no changes were observed in COS1NR and MFH1NR. The results indicated that methylation of CpG islands near a TATA box region played a critical role for gene silencing of the rat p16^INK4a^ gene, rather than that of other regions. Β© 2003 WileyβLiss, Inc.
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