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Dickinson State University INBRE Program April 2006

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Our hypothesis is that lycopene's anticarcinogenic properties ... HS-68, foreskin fibroblast cells. A549, lung carcinoma cells. HS-578T, breast carcinoma cells ... – PowerPoint PPT presentation

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Title: Dickinson State University INBRE Program April 2006


1
Dickinson State UniversityINBRE ProgramApril
2006
  • Lynn C. Burgess, Ph.D.
  • Dickinson State University, Dickinson, ND

2
Projects
  • The anticarcinogenic mechanism of lycopene
  • The pathology of exuberant granulation tissue in
    equine

3
Lycopene Hypothesis
  • Our hypothesis is that lycopenes
    anticarcinogenic properties is due to its ability
    to increase or renew gap junctional connexin
    protein expression. Therefore, lycopene
    maintains or creates gap junctional communication
    from cell to cell, which can control
    proliferation of neoplastic cells from
    surrounding normal cells.

4
Lycopene
  • To test the hypothesis that lycopenes
    anticarcinogenic property was due to suppression
    of the cancer cells proliferation.
  • We tested the following human cell lines
  • DU-145, prostate adenocarcinoma cells
  • HS-68, foreskin fibroblast cells
  • A549, lung carcinoma cells
  • HS-578T, breast carcinoma cells
  • RWPE-1, prostate cells
  • IMR-90, lung cells

5
Cell Proliferation Results
  • None of the cell lines showed any significant
    changes to their proliferation at any of their
    sample times contrary to other published reports.
    All the cells grew normally and continued to
    proliferate through the 72 hours of incubation.
  • Treated cells were compared to controls using the
    Mann-Whitney U Test

6
Lycopene and Connexin mRNAs
  • RNAs of treated cells were extracted and
    converted to cDNAs. With the use of standard
    PCR, 17 connexins mRNAs were tested for their
    expression in the cell lines
  • Connexins 26, 29, 30, 30.3, 31, 31.1, 31.9, 32
    36, 37, 40, 43, 45, 50, and 59 were expressed in
    the cells and there was no expressions from 46
    and 47 in any of the cell lines.

7
Connexin Protein Expression
  • ELISA and Western Blots are being used to test
    the changes to the connexin proteins after
    lycopene treatment

8
Experiments for Next Year
  • Three more cell lines will be added
  • QPCR will be used to measure any changes in
    connexin mRNA expression due to the lycopene
    treatments
  • The effect of lycopene on cell migration will be
    examined

9
Exuberant Granulation TissueHypothesis
  • The capillary endothelial cells from equine
    exuberant granulation tissue are self simulating
    due to the expression of VEGF and causing the
    overgrowth of the tissue
  • We also needed to culture and characterized
    capillary endothelial cells from the disorder.

10
Exuberant Granulation TissueProud Flesh
11
Endothelial Cell Culturing
  • Tissue was minced and treated with typsin then
    sparely seeded on plates. The cells were
    generally attached after 24 h.
  • The cells had a fusiform to polygonal appearance.
    They grew to a monolayer by 2 weeks and formed
    round colonies of cells that had a cobblestone
    appearance.
  • The EC appeared to be uniform in type without
    contaminating fibroblasts.
  • Growth rates of the cells increased as the
    initial seeding was cultured for the 2 weeks.
    The cells retained their appearance and continued
    to after multiple passages.
  • A immunofluorescence study confirmed the
    phenotype with an antibody to von Willebrand
    factor (factor VIII). Confluence cultures of
    showed strong cytoplasmic staining in all the
    cells

12
Growth Factors Expression in Endothelial Cells
  • mRNAs from cultured endothelial cells were tested
    with PCR for angiogenic and inflammation growth
    factor expression
  • VEGF, midkine, fibroblast growth factors a and
    ß, somastatin, platelet factor-4, thrombospondin,
    leukemia inhibitory factor, interferon ?,
    transforming growth factor-ß, and insulin-like
    growth factor-1.

13
Growth Factor Expression
  • The EC expressed two isoforms of vascular
    endothelial growth factor (VEGF) these were 121
    and 165
  • There was no expression of other angiogenic and
    inflammation growth factors

14
Exuberant Granulation TissueConclusions
  • Exuberant granulation tissue provides an easily
    cultured source of capillary EC, which should be
    valuable in studies of the disease
  • The expression of VEGF by the EC shows a
    self-simulation that may be the pathology for
    this disease
  • VEGF was the angiogenic growth factor expressed
    and could be a possible target for treatment

15
The DSU INBRE Research Group
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