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Control of Gene Expression

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Knock-out animals in which a particular gene of interest is replaced with a ... The process is based on endogenous enzymes, which must have some natural function ... – PowerPoint PPT presentation

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Title: Control of Gene Expression


1
Control of Gene Expression
2
Ways to study protein function by manipulating
gene expression
  • Mutations
  • Naturally occurring, including human and animal
    genetic diseases
  • Induced by radiation or chemical mutagenesis
  • targeted
  • Knock-out animals in which a particular gene of
    interest is replaced with a gene engineered to be
    non-functional
  • Gene knockdown in which the mRNA for a
    particular gene is interfered with or destroyed

3
For some animals, a large library of mutants has
accumulated
  • Drosophila
  • C. elegans
  • Mouse

4
animals with targeted mutations gene knockout
  • Introduce DNA fragment containing altered version
    of target gene into embryonic stem cells (ES
    cells) growing in culture
  • Separate cells and allow each to form a colony
  • Select those colonies in which the introduced
    fragment has replaced the target gene
  • Inject ES cells into 3-day blastocysts to create
    chimeric embryos
  • Implant embryos into recipient mothers
  • Resulting 1st generation animals will be chimeric
    some of them will have gonads formed from the
    introduced cells, so will be able to pass the
    altered gene on
  • Breed the 1st generation to one another to get
    transgenic animals in which the altered gene is
    present on both chromosomes these are called
    knockout animals if the replacement gene is
    non-functional

5
Disadvantages of the knockout approach
  • The target protein may be so essential that it is
    backed up by other proteins (I.e., there is
    redundancy), so the phenotype shows no impairment
  • Animals lacking the target gene may not survive
    embryonic development
  • Making knockout animals is a time-consuming and
    expensive process about 1 year and 200,000 for
    each knockout mouse line.

6
There is another way gene knockdown
  • Two methods
  • antisense RNA
  • inhibitory RNA

7
Antisense RNA
  • is single-stranded RNA complementary to the mRNA
    of the gene of interest
  • Cells take up the antisense RNA, which pairs with
    the native mRNA, interfering with its translation
    to protein

8
RNA interference
  • Generate doublestranded RNA complementary to the
    sequence of the mRNA of interest cells take
    these up.
  • An intracellular enzyme called Dicer cuts the
    dsRNA into small double and single-stranded
    fragments of 20-25 base pairs
  • Fragments associate with an RNA-induced silencing
    complex (RISC) composed of several proteins.
    This complex recognizes the mRNA containing the
    complementary sequence. One of the proteins in
    the complex (argonaute) then cleaves the mRNA
    into pieces, preventing its translation.
  • http//www.nature.com/nrg/journal/v2/n2/animation/
    nrg0201_110a_swf_MEDIA1.html

9
Disadvantages of RNA-based gene knockdown
  • Its usually temporary
  • Delivering the RNA may be problematic, depending
    on the organism sometimes it is necessary to
    infect the organism with a vector virus carrying
    the desired RNA sequence

10
RNA inhibition is a naturally-occurring process
  • The genome contains a large amount of what was
    once characterized as junk DNA we no realize
    that some of this codes for RNAi
  • The process is based on endogenous enzymes, which
    must have some natural function
  • It is also involved in viral disease, since some
    viral genomes code for RNAi that is effective
    against host cells
  • It is likely that RNAi will be a route of gene
    therapy.
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