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Transgenic and knockout mice

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Title: Transgenic and knockout mice


1
Transgenic and knockout mice
  • Dr. Sumbul Fatma

2
Mice - Models of Human Diseases
  • Although the human is the mammal we are generally
    most interested in learning more about, it is
    also the one animal we cannot use for genetic
    experiments for obvious ethical reasons
  • Mice naturally develop conditions that mimic
    human disease, such as cardiovascular disease,
    cancer and diabetes
  • Mouse are a favorite model for human disease
    because it has a relatively low cost of
    maintenance and a generation time that measures
    only nine weeks
  • Developments in molecular biology and stem cell
    biology have allowed researchers to create
    custom-made mice through gene targeting in mouse
    embryonic stem (ES) cells
  • Certain diseases that afflict only humans, such
    as cystic fibrosis and Alzheimer's can also be
    induced by manipulating the mouse genome and
    environment

3
ES Cells and Chimeric Mice
  • Embryonic stem (ES) cells are pluripotent cell
    lines with the capacity of self-renewal and a
    broad differentiation plasticity
  • They are derived from pre-implantation embryos
    and can be propagated as a homogeneous,
    uncommitted cell population for an almost
    unlimited period of time
  • Even after extensive genetic manipulation, mouse
    ES cells are able to reintegrate fully into
    viable embryos when injected into a host
    blastocyst
  • After these pre-implantation embryos are
    implanted into a surrogate mother, they develop
    into mosaic offspring known as chimeras. The
    tissues of chimeric mice are comprised of a
    mixture of cells that originated from both the
    host embryo and the ES cells.

4
Knockout Mice
  • A knockout mouse is a genetically engineered
    mouse in which one or more genes have been turned
    off through a gene knockout
  • Important animal models for studying the role of
    genes which have been sequenced, but have unknown
    functions
  • By causing a specific gene to be inactive in the
    mouse, and observing any differences from normal
    behaviour or condition, researchers can infer its
    probable function.

5
Transgenics
  • This technique permits the introduction of
    foreign genes or altered forms of an endogenous
    gene into an organism
  • Mostly, this technique does not result in
    replacement of the endogenous gene, but rather
    the integration of additional copies of it
  • The introduced gene is called transgene and the
    organism carrying it is referred to as transgenic

6
Transferring DNA into eukaryotic cells
  • Production of both knockout and transgenic
    animals requires the transfer of DNA into
    eukaryotic cells.
  • Calcium precipitation
  • Liposome delivery
  • Microinjection
  • Electroporation

7
  • Calcium phosphate precipitates of DNA form when
    DNA is mixed with calcium chloride. When these
    DNA precipitates are added to animal cells
    growing in culture, the precipitated DNA can be
    taken up by the cells, again transferred to the
    nucleus and expressed
  • Liposomes are artificial membranes that can be
    formed in a test tube. DNA can be mixed with the
    liposome preparation under the appropriate
    conditions. This results in the encapsulation of
    DNA into synthetic lipid membranes. When this
    membrane fuses with the cell plasmamembrane, DNA
    is released into the cell and somehow ends up in
    the nucleus.

8
DNA microinjection
  • DNA can also be injected directly into the nuclei
    of both cultured cells and developing embryo

9
Electroporation
  • Cells are subjected to a brief electric shock of
    several thousand volts and become transiently
    permeable to DNA. Presumably the shock briefly
    opens holes in the cell membrane allowing the DNA
    to enter the cells before the holes reseal

10
DNA incorporation in the cell
  • Once the foreign DNA is inside the host cell,
    enzymes that function normally in DNA repair and
    recombination join the fragments of foreign DNA
    into the host cells chromosome
  • The new fragment can either replace an endogenous
    gene- homologous recombination or it can remain
    as an independent extrachromosomal DNA molecule
    referred to as an episome

11
Identification of transgenic cells
  • Since only a relatively small fraction of cells
    take up DNA, a selective technique must be
    available to identify the transgenic cells
  • In most cases the exogenous DNA includes two
    additional genes
  • The small fraction of cells in which homologous
    recombination takes place can be identified by a
    combination of positive and negative selection

12
Positive and Negative selection
  • Positive Selection- One of the additional genes
    (neoR) confers neomycin resistance it permits
    positive selection of cells in which either
    homologous (specific) or non-homologous (random)
    recombination has occurred
  • Negative selection- The second gene, thymidine
    kinase gene from Herpes Simplex Virus (tkHSV)
    confers sensitivity to gancyclovir(a cytotoxic
    nucleotide analog). This gene permits negative
    selection of ES cells in which non-homologous
    recombination has occurred
  • Only ES cells that undergo homologous
    recombination (i.e. gene-targeted specific
    insertion of the DNA construct) can survive this
    selection scheme

13
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14
Positive and Negative selection of recombinant
ES cells
15
Knockout Mice
  • Gene knockout is a technique for selectively
    inactivating a gene by replacing it with a mutant
    allele in an otherwise normal organism (mice)
  • Knockout mice are a useful model system for
    studying certain human genetic diseases.

16
Making knockout mice
  • Mutant alleles are introduced by homologous
    recombination into Embryonic Stem cells
  • ES cells containing the knockout mutation are
    introduced into early mouse embryos. The
    resultant mice will be chimeras containing
    tissues derived from both the transplanted ES
    cells and host cells. These cells can contribute
    to both germ cell and somatic cell population
  • Chimeric mice are mated to assess whether the
    mutation is incorporated into the germline
  • Chimeric mice each heterozygous for the knockout
    mutation are mated to produce homozygous knockout
    mice

17
Knockout Mice to study genetic diseases
  • Knockout mice make good model systems for
    investigating the nature of genetic diseases and
    the efficacy of different types of treatment and
    for developing effective gene therapies to cure
    these often devastating diseases
  • For instance, the knockout mice for CFTR gene
    show symptoms similar to those of humans with
    cystic fibrosis

18
Transgenic animals
  • Transgenic animals carry cloned genes that have
    integrated randomly into the host genome
  • Transgenic technology has numerous experimental
    application and potential therapeutic value
  • The frequency of random integration of exogenous
    DNA into mouse genome at non-homologous sites is
    very high, therefore, the production of
    transgenic mice is a highly efficient and
    straightforward process

19
  • Foreign DNA containing a gene of interest is
    injected into one of the two pronuclei (the male
    and female nuclei contributed by the parent) of a
    fertilized mouse egg before they fuse
  • The injected DNA has a good likelihood of being
    randomly integrated into the chromosome of the
    diploid zygote

20
  • Injected eggs are then transferred to foster
    mothers in which normal cell growth and
    differentiation occurs
  • About 10-30 of progeny will contain the foreign
    DNA in equal amounts in all tissues, including
    the germ cells
  • Immediate breeding and backcrossing of these mice
    can produce pure transgenic strains homozygous
    for the transgene

21
Transgenics and gene therapy
  • Once a gene mutation is identified to be the
    cause of a disease, the next step is to cure the
    disease by introducing normal genes( transgene)
    into affected individual
  • In experimental animals, some genetic disorders
    have been cured by gene therapy, but in humans,
    numerous technical issues need to be resolved
    before it can be widely used
  • a) how to reliably and safely introduce various
    genes into human cells
  • b) tissue/ cell specific introduction of genes
  • c) large size of genes
  • d)how to address the ethical issues
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