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Transgenic Animals, Knock-Out Mice and Dolly

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Title: Transgenic Animals, Knock-Out Mice and Dolly


1
Pluripotent ES Cells
  • Pluripotent ES cells are undifferentiated early
    embryonic cells derived from the inner cell mass
    of mouse blastocysts.
  • In vitro ES cells must be grown on a feeder layer
    of fibroblasts to prevent them from
    differentiating.
  • Introduction of the transgene is achieved by
    electroporation of retroviral infection.
  • The transgene must integrate via recombination,
    not randomly.
  • Cells transfected successfully can be identified
    prior to injection into blastocysts.

2
Specific Gene Targeting in ES Cells
  • Gene targeting can be achieved using gene
    constructs designed for homologous recombination.
    This technique can be used to either
  • Knockout functional genes to study their
    contribution to different developmental or
    disease processes (null mutations)
  • Genes encoding b2m, MHC class I and II. CD2, Ii,
    TCR, Ig, IL-4, IL-2, FceR, TAP1/2, RAG-2,and many
    more (gt100)!
  • Replace a functional gene for a
    mutated/non-functional gene to restore wild type
    phenotype .
  • Gene encoding HGPRT in mice deficient for HGPRT
    (called Lesch-Nhyan syndrome in humans).

3
DNA Constructs for Recombination
  • DNA vectors contain the gene of interest which
    has been interrupted with an antibiotic
    resistance gene (hygromycin resistance, or G418
    resistance).
  • To ensure targeted integration has occurred, the
    flanking DNA contains the thymidine kinase gene.
    If TK integrates (random insertion), then the
    transfected cells die when grown in selective
    media (gancyclovir).

4
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5
Selection of Targeted ES Cells
  • Gancyclovir resistant and G418 resistant ES cells
    grow into small clumps on top of feeder cells.
  • The colonies of cells can be picked off and
    transferred to new wells (at 0.3 cells per well
    seeding density) containing feeder cells.
  • When sufficient numbers of cells are obtained,
    they are
  • Frozen for safe storage
  • Analyzed by Southern blotting or PCR to determine
    nature of integration event
  • Microinjected into the blastocoel cavity of
    blastocysts.

6
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7
  • http//www.criver.com/products/genetic_testing/dxg
    mon2.html

8
Dolly and the Advancement of Animal Cloning
9
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