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Träfflista för sökning "swepub ;lar1:(umu);srt2:(1990-1994);srt2:(1991);pers:(Wanders A)"

Search: swepub > Umeå University > (1990-1994) > (1991) > Wanders A

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1.
  • Wanders, A., et al. (author)
  • Evidence that LS-2616 (linomide) causes acute rejection of rat allografts protected by cyclosporine but not of long-term surviving allografts
  • 1991
  • In: Transplantation. - 0041-1337 .- 1534-6080. ; 52:2, s. 234-8
  • Journal article (peer-reviewed)abstract
    • The immunomodulator LS-2616 (Linomide) induces rejection of cyclosporine-protected rat cardiac allografts. The aim of this study was to characterize this rejection in the presence of CsA and to test LS-2616 in other models of permanent graft acceptance in the rat. PVG rat hearts were transplanted heterotopically to Wistar/Kyoto (Wi/Ky) rat recipients on day 0. The recipients were treated orally on days 0-9 with CsA (10-40 mg/kg) and/or with LS-2616 (2.5-160 mg/kg) starting at different times (day -7 -+5) until the day of complete rejection. The addition of LS-2616 (day -1--stop) to CsA (10 mg/kg) resulted in a dose-dependent antagonism of the immunosuppressive effect of CsA with daily doses of 2.5-160 mg/kg. Furthermore, the results were similar, irrespective of whether LS-2616 treatment (160 mg/kg) was started on day -7, -1, +1, +3, or +5. LS-2616 (160 mg/kg) pretreatment of the recipient for 7 days before transplantation was considerably less effective. CsA (20 mg/kg) for 14 days after a PVG to DA transplantation resulted in permanent graft survival. This was not abrogated by LS-2616. Neither was rejection induced in long-term surviving grafts of RT1.C incompatible Lewis recipients. Our data suggest that LS-2616 activates already stimulated and sensitized T cells that are otherwise controlled by CsA.
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2.
  • Dallman, M. J., et al. (author)
  • Cytokine gene expression : analysis using northern blotting, polymerase chain reaction and in situ hybridization
  • 1991
  • In: Immunol Rev. ; 119, s. 163-79
  • Journal article (peer-reviewed)abstract
    • We describe here the use of northern blotting, PCR and in situ hybridization for the analysis of cytokine gene expression. These techniques, each with their advantages and disadvantages, have been used to monitor cytokine gene expression in sites of immune reactivity and in the developing thymus. Whilst expression of a gene usually correlates well with protein production from that gene, this may not always be the case. The development of methods to analyze protein production in situ, for instance by immunohistochemistry, together with analysis of mRNA expression will allow us to begin to understand the role of cytokines within the immune system of the intact animal.
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  • Result 1-3 of 3
Type of publication
journal article (3)
Type of content
peer-reviewed (3)
Author/Editor
Larsson, E (1)
Gerdin, Bengt, 1947- (1)
Fellstrom, B (1)
Tufveson, G (1)
Dimeny, E (1)
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Karlsson-Parra, A (1)
Dallman, M. J. (1)
Montgomery, R. A. (1)
Larsen, C. P. (1)
Wells, A. F. (1)
Vogt, P. (1)
Foegh, M. L. (1)
Tufvesson, G. (1)
Wonigkeit, K. (1)
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University
Uppsala University (1)
Language
English (3)
Research subject (UKÄ/SCB)
Medical and Health Sciences (3)
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