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Genetic engineering of animal cells in culture To study individual genes, it may be necessary to transfer the gene into the cells under study.  In this section we will discuss some of the common methods that are used to introduce genes into mammalian cells.  This is essential so that one can genetically manipulate cells  so that they are able to produce large levels of the desired protein (overexpression). In the diagram, a gene is spliced into a plasmid, called shuttle vectors, and then introduced into the mammalian cell.
Outline ,[object Object],[object Object],[object Object],[object Object],[object Object]
Lecture 7 Animal Cell Biotechnology Genetic engineering of animal cells ,[object Object],[object Object],[object Object],[object Object],[object Object]
Lecture 7 Animal Cell Biotechnology Genetic engineering of animal cells ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
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2.  DEAE-dextran ,[object Object],[object Object],[object Object]
3.  Encapsulation of DNA in liposome vesicles (lipofection) ,[object Object],[object Object],[object Object],[object Object]
 
4.  Electroporation ,[object Object],[object Object],[object Object],[object Object],[object Object],http://www.youtube.com/watch?v=s0zM-3dmO4M http://aditusmedical.com/
5.  Micro-injection ,[object Object],[object Object],http://www.youtube.com/watch?v=h-Bfc1GPWpE
6.  Protoplast fusion ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
Lecture 7 Animal Cell Biotechnology Genetic engineering of animal cells ,[object Object],[object Object],[object Object],[object Object],[object Object],[object Object]
Simian virus SV40   ,[object Object],[object Object],[object Object],[object Object]
Retroviruses ,[object Object],[object Object],[object Object],[object Object]
 
Selection  and  amplification  of transfected cells ,[object Object],[object Object],[object Object],[object Object]
Genetic markers… ,[object Object],[object Object],[object Object],eg. Glutamine synthetase: amplified by addition of methionine sulfoximine
[object Object],[object Object],[object Object]
[object Object],[object Object],[object Object],[object Object],[object Object],Simple Precursors:  purine, pyrimidine and nucleotides DNA Hypoxanthine  or  Guanine Thymidine TK HGPRT Salvage  pathway Aminopterin inhibition De novo  pathway
Genetic Markers… ,[object Object],eg.  Xanthine-Guanine Phosphoribosyl transferase (XGPRT)   -present only in bacteria naturally -only transfected mammalian cells would be able to survive in media with xanthine, hypoxanthine mycophenolic acid
3. antibiotic resistance genes ,[object Object],[object Object]
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[object Object],[object Object],[object Object],Gene expression ,[object Object]
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Expression cassettes ,[object Object],[object Object],[object Object]
Signal sequences of an expression cassette include: ,[object Object],[object Object],[object Object],[object Object]
Lecture 7 Animal Cell Biotechnology   Genetic engineering of animal cells ,[object Object],[object Object],[object Object],[object Object],Butler, M.  2004.  Animal cell culture and technology 2nd ed. London and New York:Garland Science/BIOS Scientific Publishers. P106.

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Lecture 8 genetic engineering of animal cells

  • 1. Genetic engineering of animal cells in culture To study individual genes, it may be necessary to transfer the gene into the cells under study. In this section we will discuss some of the common methods that are used to introduce genes into mammalian cells. This is essential so that one can genetically manipulate cells so that they are able to produce large levels of the desired protein (overexpression). In the diagram, a gene is spliced into a plasmid, called shuttle vectors, and then introduced into the mammalian cell.
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Hinweis der Redaktion

  1. To study individual genes, it may be necessary to transfer the gene into the cells under study. In this section we will discuss some of the common methods that are used to introduce genes into mammalian cells. This is essential so that one can genetically manipulate cells so that they are able to produce large levels of the desired protein (overexpression). In the diagram, a gene is spliced into a plasmid, called shuttle vectors, and then introduced into the mammalian cell.
  2. CHO cells are very popular for the expression of human recombinant glycoproteins because the glycosylation enzymes resemble those found in human cell lines. They can grow as anchorage dependent or as cell suspensions.
  3. Introduction of DNA into cells with commercially available cationic lipids. Charged head groups (positive) are drawn to the phosphate backbone of DNA.
  4. Electroporation Exposure of suspended cells to a pulsed electric field that causes the transient formation of pores in the cell membrane, allowing for exchange of macromolecules between the extracellular environment and the cytoplasm. Removal of the electrical field results in spontaneous sealing of the pores. Microinjection DNA injected with microneedles or pipettes directly into the nucleus, or into the cytoplasm. Requires highly trained and skilled personnel. Typically used when there are limited numbers of recipient cells.
  5. Bacteria are used to produce plasmids containing the human gene of interest. The cell walls are removed using lysozyme, resulting in the formation of protoplasts. The protoplasts are brought in contact with the mammalian cells, leading to protoplast fusion to mammalian cells, using Polyethylene glycol (PEG).
  6. Overview of methods discussed, in handout.
  7. Non-dominant genes: target cells must have endogenous genes mutated or removed, only works with mutant cells. If target genes are successfully transfected with shuttle vector containing wild-type marker gene, this will allow cells to survive in specially treated media. Dominant genes: do not require mutant cells, can be used with any cell type. Dominant marker genes do not have to be mammalian, may be bacterial in origin, allows the cell to survive in special medium. Antibiotic resistance genes: shuttle vector contains antibiotic, allows for successful transfectants to survive.