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INFLAMMATION IN ALZHEIMER DISEASE: EFFECTS OF
                               CANNABINOIDS
                                                      Diana Aguirre-Rueda and Soraya L. Valles
                                      Department of Physiology, School of Medicine, University of Valencia, Spain.

  Introduction


The hallmark in Alzheimer’s disease (AD) is both accumulation of beta-amyloid (Aβ) plates and the presence of TAU protein inside
neurons. Furthermore, glial cell activation, occurs after plates appear in brain damaged producing astrogliosis and microglia activation.
Our group has shown inflammation in astrocytes in primary culture comparing Aβ with control cells. Here we determined the action of
cannabinoids in Aβ inflammation in astrocytes in culture. Protein expression levels were detected by ELISA and Western- blot techniques
in astrocytes in primary culture treated with Aβ and/or cannabinoids. Using Aβ (10 μM) during 24 h, an increase of pro-inflammatory
mediators (TNF-α and IL-1β), compared with control astrocytes was detected. Treatment with Win 55, 212-2 (10 μM) produced increase
of anti-inflammatory mediators (PPAR-γ) and decrease of pro-inflammatory mediators, such as TNF-α and IL-1β, protecting cells to the
toxic effect of Aβ.

    (C )                       (Aβ)                     (WIN)                   (WIN + Aβ )


                                                                                                           Fig. 1.- Confocal microscopy. Treated
                                                                                                           cells for 24 h with 10 μM Aβ (40-1) (C),
                                                                                                           10 μM Aβ (1-42) (Aβ), 10 μM WIN 55,
                                                                                                           212-2 (WIN) and 10 μM Aβ (1-42) + 10
                                                                                                           μM WIN 55, 212-2 (WIN+Aβ ).




    Fig. 1. IL-1β levels in astrocytes in primary culture. IL-1β levels were    Fig. 2. TNF-α levels in astrocytes in primary culture. TNF-α levels were
    determined by ELISA in astrocytes treated for 24 h with 10 μM Aβ (40-1)     determined by ELISA in astrocytes treated for 24 h with 10 μM Aβ (40-1) (C), 10
    (C), 10 μM Aβ (1-42) (Aβ), 10 μM WIN 55, 212-2 (WIN) and 10 μM Aβ (1-       μM Aβ (1-42) (Aβ), 10 μM WIN 55, 212-2 (WIN) and 10 μM Aβ (1-42) + 10 μM
    42) + 10 μM WIN 55, 212-2 (Aβ + WIN). Data are mean ± D.S. * p < 0.05       WIN 55, 212-2 (Aβ + WIN). Data are mean ± D.S. * p < 0.05 vs control cells # p
    vs control cells # p < 0,05 vs Aβ treated cells. n = 3.                     < 0,05 vs Aβ treated cells. n = 3.




                                      Fig. 4. PPAR-γ expression in astrocytes in primary culture. PPAR-γ expression were
                                      determined by western-blot in astrocytes treated for 24 h with 10 μM Aβ (40-1) (C), 10
                                      μM Aβ (1-42) (Aβ), 10 μM WIN 55, 212-2 (WIN) and 10 μM Aβ (1-42) + 10 μM WIN 55,
                                      212-2 (Aβ + WIN). Data are mean ± D.S. * p < 0.05 vs control cells # p < 0,05 vs Aβ
                                      treated cells. n = 3.


                                                                        CONCLUSION

     These results demonstrate an unbalance between inflammatory and anti-inflammatory mediators in Alzheimer’s disease and
     suggest that Aβ is able to induce inflammation in astrocytes and this effect are prevented by cannabinoids as a possible positive
     effect in AD.

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Poster congreso madrid 2012 pdf

  • 1. INFLAMMATION IN ALZHEIMER DISEASE: EFFECTS OF CANNABINOIDS Diana Aguirre-Rueda and Soraya L. Valles Department of Physiology, School of Medicine, University of Valencia, Spain. Introduction The hallmark in Alzheimer’s disease (AD) is both accumulation of beta-amyloid (Aβ) plates and the presence of TAU protein inside neurons. Furthermore, glial cell activation, occurs after plates appear in brain damaged producing astrogliosis and microglia activation. Our group has shown inflammation in astrocytes in primary culture comparing Aβ with control cells. Here we determined the action of cannabinoids in Aβ inflammation in astrocytes in culture. Protein expression levels were detected by ELISA and Western- blot techniques in astrocytes in primary culture treated with Aβ and/or cannabinoids. Using Aβ (10 μM) during 24 h, an increase of pro-inflammatory mediators (TNF-α and IL-1β), compared with control astrocytes was detected. Treatment with Win 55, 212-2 (10 μM) produced increase of anti-inflammatory mediators (PPAR-γ) and decrease of pro-inflammatory mediators, such as TNF-α and IL-1β, protecting cells to the toxic effect of Aβ. (C ) (Aβ) (WIN) (WIN + Aβ ) Fig. 1.- Confocal microscopy. Treated cells for 24 h with 10 μM Aβ (40-1) (C), 10 μM Aβ (1-42) (Aβ), 10 μM WIN 55, 212-2 (WIN) and 10 μM Aβ (1-42) + 10 μM WIN 55, 212-2 (WIN+Aβ ). Fig. 1. IL-1β levels in astrocytes in primary culture. IL-1β levels were Fig. 2. TNF-α levels in astrocytes in primary culture. TNF-α levels were determined by ELISA in astrocytes treated for 24 h with 10 μM Aβ (40-1) determined by ELISA in astrocytes treated for 24 h with 10 μM Aβ (40-1) (C), 10 (C), 10 μM Aβ (1-42) (Aβ), 10 μM WIN 55, 212-2 (WIN) and 10 μM Aβ (1- μM Aβ (1-42) (Aβ), 10 μM WIN 55, 212-2 (WIN) and 10 μM Aβ (1-42) + 10 μM 42) + 10 μM WIN 55, 212-2 (Aβ + WIN). Data are mean ± D.S. * p < 0.05 WIN 55, 212-2 (Aβ + WIN). Data are mean ± D.S. * p < 0.05 vs control cells # p vs control cells # p < 0,05 vs Aβ treated cells. n = 3. < 0,05 vs Aβ treated cells. n = 3. Fig. 4. PPAR-γ expression in astrocytes in primary culture. PPAR-γ expression were determined by western-blot in astrocytes treated for 24 h with 10 μM Aβ (40-1) (C), 10 μM Aβ (1-42) (Aβ), 10 μM WIN 55, 212-2 (WIN) and 10 μM Aβ (1-42) + 10 μM WIN 55, 212-2 (Aβ + WIN). Data are mean ± D.S. * p < 0.05 vs control cells # p < 0,05 vs Aβ treated cells. n = 3. CONCLUSION These results demonstrate an unbalance between inflammatory and anti-inflammatory mediators in Alzheimer’s disease and suggest that Aβ is able to induce inflammation in astrocytes and this effect are prevented by cannabinoids as a possible positive effect in AD.