5 Stages involved in GE Isolation Cutting Ligation and Insertion

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5 Stages involved in GE Isolation Cutting Ligation and Insertion

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Presentation transcript:

5 Stages involved in GE Isolation Cutting Ligation and Insertion Transformation Cloning & Expression

1. Isolation (a) Isolation of a specific gene from donor e.g. human Cells broken open Genetic probe added Reveals position of the gene of interest The first step involves breaking open the cells of the donor to release the DNA and isolate the gene of interest e.g. insulin producing gene. Cells are broken open using chemicals and enzymes e.g. washing up liquid Donor DNA is extracted Genetic probe is added A DNA probe consists of a small fragment of DNA labelled with an enzyme, a radioactive tag or a flurescent dye tag. The probe will bind to a complementary DNA sequence by base pairing. Identifying the presence and location of the gene of interest Genetic probe Position of gene of interest Donor DNA

1. Isolation (b) Isolation of plasmid from a bacterial cell The DNA from the bactterial cell is released. A bacterial cell contains a circular loop of DNA called a plasmid. The plasmid is isolated from the bacterial cell. The plasmid will act as a vector for carrying a new gene i.e. the gene from the donor will be inserted into the plasmid DNA.. www.sci.sdsu.edu

2. Cutting Human DNA and plasmid DNA are cut open using the same restriction enzymes The donor DNA and plasmid DNA are cut using enzymes called restriction enzymes. Restriction enzymes recognise specific sequence of bases Act as a molecular scissors to cut the DNA strand within the recognition sequence. The donor DNA and plasmid DNA are cut using the same restriction enzymes. Bacteria use restriction enzymes to defend themselves against attacks from bacterial viruses. The enzymes cut invading viral DNA and render it harmless.

3. Ligation The target gene is placed in the DNA of the plasmid/cloning vector and joins on to it When cut plasmids are mixed with cut human DNA, different combinations result. DNA ligase is used to form strong bonds within the recombinant DNA

2. Cutting & 3. Ligation

4. Transformation Uptake of recombinant DNA into cell Vast majority of cells Some cells Some cells Special techniques will identify the small number of bacteria with the target gene

4. Transformation

5. Cloning & Gene Expression Cloning: Identical copies of the bacteria with the target gene are produced Universality of genetic code Plasmid will produce the polypeptide coded for by the donor DNA Expression: Getting the organism with the recombinant DNA to produce the desired protein