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ANTIINFLAMMATORY EFFECTS OF JOBELYN Phase I Results

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Ferdinand-Porsche Str. 5, D 79211 Denzlingen, Germany and it's Affiliates with ... Effects of Jobelyn on lipopolysaccharide(LPS)-induced cytokine, and PGE2 release ... – PowerPoint PPT presentation

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Title: ANTIINFLAMMATORY EFFECTS OF JOBELYN Phase I Results


1
ANTI-INFLAMMATORY EFFECTS OF JOBELYN(Phase I
Results)
  • PREPARED BY
  • VIVACELL BIOTECHNOLOGY GMBH,
  • Ferdinand-Porsche Str. 5,
  • D 79211 Denzlingen, Germany and its
    Affiliates with
  • offices at Freiburg, Germany and VivaCell,
    Córdoba, Spain
  • Dr. Bernd Fiebich
  • VivaCell Technologies GmbH
  • AND
  • Dr. Kurt Appel
  • VivaCell Technologies GmbH

2
Anti-inflammatory effects of Jobelyn
  • Effects of Jobelyn on lipopolysaccharide(LPS)-indu
    ced cytokine, and PGE2 release in human monocytes
  • Human primary monocytes were isolated from buffy
    coats of healthy human blood donors.
  • Cells were seeded in 24-well plates for ELISA
    measurements.
  • Monocytes were incubated without or with LPS (10
    ng/ml) for 24 h in absence or presence of Jobelyn
    (6 doses 1, 10, 50, 100, 250, and 500 µg/ml
    depending on cytotoxicity), which were added 30
    min before LPS treatment.
  • After 24 h (with or without LPS), supernatants
    were removed, centrifuged and investigated for
    cytokines (IL-1beta, TNFalpha, IL-6, IL-8), and
    PGE2 concentrations in ELISA using manufacturers
    protocol.

3
IL-8 ( of LPS control)
JOBELYN 1 µg/ml
LPS (10 ng/ml)
JOBELYN 10 µg/ml
JOBELYN 100 µg/ml
JOBELYN 250 µg/ml
JOBELYN 500 µg/ml
Figure 1 Inhibitory effects of JOBELYN on
LPS-induced release of IL-8 in primary human
monocytes (n3). Monocytes were pre-incubated
with JOBELYN in the indicated concentrations for
30 min and subsequently treated with LPS (10
ng/ml) for 24 h. IL-8 in the supernatants was
measured using an enzyme immunoassay (ELISA).
4
IL-1 ( of LPS control)
JOBELYN 1 µg/ml
LPS (10 ng/ml)
JOBELYN 10 µg/ml
JOBELYN 100 µg/ml
JOBELYN 250 µg/ml
JOBELYN 500 µg/ml
Figure 2 Inhibitory effects of JOBELYN on
LPS-induced release of IL-1beta in primary human
monocytes (n3). Monocytes were pre-incubated
with JOBELYN in the indicated concentrations for
30 min and subsequently treated with LPS (10
ng/ml) for 24 h. IL-1beta in the supernatants was
measured using an enzyme immunoassay (ELISA).
5
TNF ( of LPS control)
JOBELYN 1 µg/ml
LPS (10 ng/ml)
JOBELYN 10 µg/ml
JOBELYN 100 µg/ml
JOBELYN 250 µg/ml
JOBELYN 500 µg/ml
Figure 3 Inhibitory effects of JOBELYN on
LPS-induced release of TNFalpha in primary human
monocytes (n3). Monocytes were pre-incubated
with JOBELYN in the indicated concentrations for
30 min and subsequently treated with LPS (10
ng/ml) for 24 h. TNFalpha in the supernatants was
measured using an enzyme immunoassay (ELISA).
6
IL-6 ( of LPS control)
JOBELYN 1 µg/ml
LPS (10 ng/ml)
JOBELYN 10 µg/ml
JOBELYN 100 µg/ml
JOBELYN 250 µg/ml
JOBELYN 500 µg/ml
Figure 4 Inhibitory effects of JOBELYN on
LPS-induced release of IL-6 in primary human
monocytes (n3). Monocytes were pre-incubated
with JOBELYN in the indicated concentrations for
30 min and subsequently treated with LPS (10
ng/ml) for 24 h. IL-6 in the supernatants was
measured using an enzyme immunoassay (ELISA).
7
PGE2 ( of LPS control)
JOBELYN 1 µg/ml
LPS (10 ng/ml)
JOBELYN 10 µg/ml
JOBELYN 100 µg/ml
JOBELYN 250 µg/ml
JOBELYN 500 µg/ml
Figure 5 Inhibitory effects of JOBELYN on
LPS-induced release of PGE2 in primary human
monocytes (n2 on LPS-induced release of PGE2 in
primary human monocytes (n2). Monocytes were
pre-incubated with JOBELYN in the indicated
concentrations for 30 min and subsequently
treated with LPS (10 ng/ml) for 24 h. PGE2 in the
supernatants was measured using an enzyme
immunoassay (EIA).
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