Selection of Insulinoma Cell Lines With Resistance to Interleukin-1 – and -Interferon–Induced Cytotoxicity

نویسندگان

  • Guoxun Chen
  • Hans E. Hohmeier
  • Rosa Gasa
  • Veronique Vien Tran
  • Christopher B. Newgard
چکیده

Engineered insulinoma cell lines may represent an alternative to isolated islets for transplantation therapy of type 1 diabetes. Success of this approach may require development of cell lines that can withstand cytokine-mediated damage. To this end, we have cultured INS-1 insulinoma cells in increasing concentrations of interleukin-1 ( I L-1 ) + -interferon (IFN) , with approximate weekly iterations over an 8-week period. Based on the C,N diphenyl-N [ 4 , 5 d i m e t h y lthiazol-2-yl]-2,5-diphenyltetrazolium bromide (MTT) viability assay, the selected cells, termed INS-1r e s, were 100% viable after 5 days of treatment with 10 ng/ml of I L-1 . These cells were also 78 ± 1.2% viable after 5 days of exposure to the combination of 10 ng/ml IL-1 and 100 U/ml IFN, whereas parental INS-1 cells treated in the same manner were only 0.3 ± 0.03% viable. INS-1r e s cells were also resistant to treatment with supernatants from activated rat peripheral blood mononuclear cells, whereas only 20% of parental INS-1 cells survived such treatment. The resistance to IL-1 conferred by this procedure was stable, whereas the partial resistance to IFNwas transient but reinducible by culture in the presence of cytokines. Stable transfection of INS-1r e s cells with a plasmid containing the human insulin cDNA and expansion of the transfected colonies in the absence of cytokines produced cell lines that were on average more resistant to I L-1 + IFN( 5 3 ± 11%) than similarly transfected clones derived from parental INS-1 cells (15 ± 7%). I m p o r t a n t l y, several INS-1r e s–derived clones retained the capacity to secrete insulin in response to glucose concentrations over the normal physiological range. With regard to the mechanism by which selection was conferred, we found normal levels of IFNr e c e p t o r mRNA, but a 60% reduction in expression of the IL-1 receptor type I (IL-1RI) in INS-1r e s cells compared with parental INS-1 cells. IL-1 signaling through p38 MAP kinase was found to be normal in INS-1r e s cells, suggesting that their expression of IL-1RI is sufficient to maintain cytokine action. However, normal IL-1 – m e d iated translocation of NF-kB and induction of inducible nitric oxide synthase expression and nitric oxide production was severely impaired in the INS-1r e s cell lines, suggesting a mechanism for the IL-1 resistance. In sum, this study defines a strategy for isolation of cytokine-resistant -cell lines and provides a new system for studying the mechanisms by which such resistance can be achieved. D i a b e t e s 4 9 :5 6 2–570, 2000

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تاریخ انتشار 2000