Translational Therapeutics

British Journal of Cancer (2007) 96, 457–463. doi:10.1038/sj.bjc.6603559 www.bjcancer.com
Published online 16 January 2007

Gemcitabine chemoresistance and molecular markers associated with gemcitabine transport and metabolism in human pancreatic cancer cells

Y Nakano1, S Tanno2, K Koizumi1, T Nishikawa1, K Nakamura1, M Minoguchi1, T Izawa1, Y Mizukami1, T Okumura2 and Y Kohgo1

  1. 1Third Department of Internal Medicine, Asahikawa Medical College, Asahikawa, Japan
  2. 2Department of General Medicine, Asahikawa Medical College, Asahikawa, Japan

Correspondence: Dr S Tanno, E-mail: tanno1se@asahikawa-med.ac.jp

Revised 6 November 2006; Accepted 22 November 2006; Published online 16 January 2007.

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Abstract

To identify predictive molecular markers for gemcitabine resistance, we investigated changes in the expression of four genes associated with gemcitabine transport and metabolism during the development of acquired gemcitabine resistance of pancreatic cancer cell lines. The expression levels of human equilibrative nucleoside transporter-1 (hENT1), deoxycytidine kinase (dCK), RRM1, and RRM2 mRNA were analysed by real-time light cycler-PCR in various subclones during the development of acquired resistance to gemcitabine. Real-time light cycler-PCR demonstrated that the expression levels of either RRM1 or RRM2 progressively increased during the development of gemcitabine resistance. Expression of dCK was slightly increased in cells resistant to lower concentrations of gemcitabine, but was decreased below the undetectable level in higher concentration-resistant subclones. Expression of hENT1 was increased in the development of gemcitabine resistance. As acquired resistance to gemcitabine seems to correlate with the balance of these four factors, we calculated the ratio of hENT1 times dCK/RRM1 times RRM2 gene expression in gemcitabine-resistant subclones. The ratio of gene expression decreased progressively with development of acquired resistance in gemcitabine-resistant subclones. Furthermore, the expression ratio significantly correlated with gemcitabine sensitivity in eight pancreatic cancer cell lines, whereas no single gene expression level correlated with the sensitivity. These results suggest that the sensitivity of pancreatic cancer cells to gemcitabine is determined by the ratio of four factors involved in gemcitabine transport and metabolism. The ratio of the four gene expression levels correlates with acquired gemcitabine-resistance in pancreatic cancer cells, and may be useful as a predictive marker for the efficacy of gemcitabine therapy in pancreatic cancer patients.

Keywords:

pancreatic cancer, ribonucleotide reductase, deoxycytidine kinase, nucleoside transporter, gemcitabine resistance, predictive marker