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Presented by Rufia Abbas
Recombinant DNA technology
Recombinant DNA technology
DNA molecules that are extracted from different
sources and chemically joined together; for example
DNA comprising an animal gene may be recombined
with DNA from a bacterium.
This method can be used to combine DNA from
different species or to create genes with new
functions. The resulting copies are called
recombinant DNA.
2
Discovery of recombinant DNA
technology
Discovery of DNA structure Watson & Crick in 1953
Isolation of DNA ligase in 1967
Isolation of REase in 1970
Paul Berg generated rDNA technology in 1972
Cohen & Boyer in 1973 produced first plasmid vector
capable of being replicated within a bacterial host
3
Goals of recombinant DNA technology
• To isolate and characterize a gene
• To make desired alterations in one or more isolated genes
• To return altered genes to living cells
• Artificially synthesize new gene
• Alternating the genome of an organism
• Understanding the hereditary diseases and their cure
• Improving human genome
4
Procedure of making rDNA
Isolating of DNA
Cutting of DNA
Joining of DNA
Amplifying of DNA
5
Isolating of DNA 6
Cutting of DNA
• DNA can be cut into large fragments by mechanical
shearing.
• Restriction enzymes are the scissors of molecular
genetics.
The Agarose Gel electrophoresis technology
display the restriction enzyme digestion
progress.
7
Joining DNA 8
Amplifying the recombinant DNA
• Transforming the recombinant DNA into a bacterial host strain.
• The cells are treated with CaCl2
• DNA is added
• Cells are heat shocked at 42 C
• DNA goes into cell by a somewhat unknown mechanism.
• Once in a cell, the recombinant DNA will be replicated.
• When the cell divides, the replicated recombinant molecules go to both
daughter cells which themselves will divide later. Thus, the DNA is
amplified
9
Vectors used in rDNA technology
• A vector is an area of DNA that can join another DNA
part without losing the limit for self-replication
• Should be capable of replicating in host cell
• Should have convenient RE sites for inserting DNA of
interest
• Should have a selectable marker to indicate which
host cells received recombinant DNA molecule
• Should be small and easy to isolate
10
Vectors used in rDNA technology
BACS
YACS
plasmid
vectors
cosmid
Lamda
phage
express
ion
11
Applications of rDNA technology
• Agriculture: growing crops of your choice (GM food),
pesticide resistant crops, fruits with attractive colors, all
being grown in artificial conditions
• Pharmacology: artificial insulin production, drug delivery to
target sites
• Medicine: gene therapy, antiviral therapy, vaccination,
synthesizing clotting factors
• Other uses:fluorescent fishes, glowing plants etc
12
References
• Campbell, Neil A. & Reece, Jane B.. (2002). Biology (6th ed.). San
Francisco: Addison Wesley.
• Peter Walter; Alberts, Bruce; Johnson, Alexander S.; Lewis, Julian; Raff,
Martin C.; Roberts, Keith (2008).
• Berg, Jeremy Mark; Tymoczko, John L.; Stryer, Lubert (2010).
• Russell, David W.; Sambrook, Joseph (2001). Cold Spring Harbor, N.Y:
Cold Spring Harbor Laboratory.
• Hannig, G.; Makrides, S. (1998). "Strategies for optimizing heterologous
protein expression in Escherichia coli".
• Mahmoudi Gomari, Mohammad; Saraygord-Afshari, Neda;
Farsimadan, Marziye; Rostami, Neda; Aghamiri, Shahin; Farajollahia,
Mohammad M. (1 December 2020).
• Brondyk, W. H. (2009). "Guide to Protein Purification, 2nd Edition.
13
14

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Recombinant DNA technology

  • 1. 1 Presented by Rufia Abbas Recombinant DNA technology
  • 2. Recombinant DNA technology DNA molecules that are extracted from different sources and chemically joined together; for example DNA comprising an animal gene may be recombined with DNA from a bacterium. This method can be used to combine DNA from different species or to create genes with new functions. The resulting copies are called recombinant DNA. 2
  • 3. Discovery of recombinant DNA technology Discovery of DNA structure Watson & Crick in 1953 Isolation of DNA ligase in 1967 Isolation of REase in 1970 Paul Berg generated rDNA technology in 1972 Cohen & Boyer in 1973 produced first plasmid vector capable of being replicated within a bacterial host 3
  • 4. Goals of recombinant DNA technology • To isolate and characterize a gene • To make desired alterations in one or more isolated genes • To return altered genes to living cells • Artificially synthesize new gene • Alternating the genome of an organism • Understanding the hereditary diseases and their cure • Improving human genome 4
  • 5. Procedure of making rDNA Isolating of DNA Cutting of DNA Joining of DNA Amplifying of DNA 5
  • 7. Cutting of DNA • DNA can be cut into large fragments by mechanical shearing. • Restriction enzymes are the scissors of molecular genetics. The Agarose Gel electrophoresis technology display the restriction enzyme digestion progress. 7
  • 9. Amplifying the recombinant DNA • Transforming the recombinant DNA into a bacterial host strain. • The cells are treated with CaCl2 • DNA is added • Cells are heat shocked at 42 C • DNA goes into cell by a somewhat unknown mechanism. • Once in a cell, the recombinant DNA will be replicated. • When the cell divides, the replicated recombinant molecules go to both daughter cells which themselves will divide later. Thus, the DNA is amplified 9
  • 10. Vectors used in rDNA technology • A vector is an area of DNA that can join another DNA part without losing the limit for self-replication • Should be capable of replicating in host cell • Should have convenient RE sites for inserting DNA of interest • Should have a selectable marker to indicate which host cells received recombinant DNA molecule • Should be small and easy to isolate 10
  • 11. Vectors used in rDNA technology BACS YACS plasmid vectors cosmid Lamda phage express ion 11
  • 12. Applications of rDNA technology • Agriculture: growing crops of your choice (GM food), pesticide resistant crops, fruits with attractive colors, all being grown in artificial conditions • Pharmacology: artificial insulin production, drug delivery to target sites • Medicine: gene therapy, antiviral therapy, vaccination, synthesizing clotting factors • Other uses:fluorescent fishes, glowing plants etc 12
  • 13. References • Campbell, Neil A. & Reece, Jane B.. (2002). Biology (6th ed.). San Francisco: Addison Wesley. • Peter Walter; Alberts, Bruce; Johnson, Alexander S.; Lewis, Julian; Raff, Martin C.; Roberts, Keith (2008). • Berg, Jeremy Mark; Tymoczko, John L.; Stryer, Lubert (2010). • Russell, David W.; Sambrook, Joseph (2001). Cold Spring Harbor, N.Y: Cold Spring Harbor Laboratory. • Hannig, G.; Makrides, S. (1998). "Strategies for optimizing heterologous protein expression in Escherichia coli". • Mahmoudi Gomari, Mohammad; Saraygord-Afshari, Neda; Farsimadan, Marziye; Rostami, Neda; Aghamiri, Shahin; Farajollahia, Mohammad M. (1 December 2020). • Brondyk, W. H. (2009). "Guide to Protein Purification, 2nd Edition. 13
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