Amplification of Ki-ras and elevation of MAP kinase activity during mammary tumor progression in C3(1)/SV40 Tag transgenic mice

  • Min Ling Liu
  • , Friederike C. Von Lintig
  • , Marek Liyanage
  • , Masa Aki Shibata
  • , Cheryl L. Jorcyk
  • , Thomas Ried
  • , Gerry R. Boss
  • , Jeffrey E. Green

Research output: Contribution to journalArticlepeer-review

40 Scopus citations

Abstract

We have previously documented that transgenic mice expressing SV40 Tag regulated by the rat prostatic steroid-binding protein C3(1) 5'-flanking region display multistage mammary tumorigenesis. To delineate genetic changes associated with mammary tumor progression, comparative genomic hybridization (CGH) was performed. CGH revealed a consistent gain of the telomeric region of chromosome 6. This region contains the Ki-ras proto-oncogene. Analyses of genomic DNA by Southern blot demonstrated up to 40-fold amplification of the Ki-ras gene. Ki-ras amplification was detected in 12, 46 and 68% of tumors from 4, 5 and 6 month old mice, respectively, whereas no amplifications were found in any preneoplastic mammary tissues. Tumors bearing Ki-ras gene amplification exhibited high levels of Ki-ras RNA and protein. The over-expressed Ki-Ras protein in these tumors appeared functionally active as indicated by the elevated MAP kinase activity. These data demonstrate that while Ki-ras amplification might not be an early event, there is a strong association between Ki-ras amplification and over-expression and mammary tumor progression in this model. This study also shows that CGH is a powerful and useful technique for identifying copy number changes during tumor progression, and that this model may provide a predictable in vivo system for studying gene amplification.

Original languageEnglish
Pages (from-to)2403-2411
Number of pages9
JournalOncogene
Volume17
Issue number18
DOIs
StatePublished - 5 Nov 1998

Keywords

  • CGH
  • Gene amplification
  • Ki-ras
  • Mammary gland tumor
  • MAP kinase
  • Ras-bound GTP and GDP
  • Transgenic mice

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