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Part 3
Mutagen
    Gene
  transfer

             Genetic
             recombi
              nation




Selection of mutants
Recombinant DNA technology, gene cloning
•   Genetic engineering involves changing
    the genetic material in an organism to
    alter its traits or products

•   A recombinant DNA molecule contains
    DNA fragments spliced together from 2 or
    more organisms
   Stages of cloning experiment
   Elements:
     Vectors
     Restriction enzymes
     Mechanism in joining the fragments
     Selection or detection of successful cloning
   Gene library
1. Joining
                  DNA segment




         Vector   2. Providing
                  milieu that
                  allows
                  propagation

Clones
1.   Remove bacterial DNA (plasmid).
2.   Cut the Bacterial DNA with
     “restriction enzymes”.
3.   Cut the DNA from another
     organism with “restriction
     enzymes”.
4.   Combine the cut pieces of DNA
     together with another enzyme and
     insert them into bacteria.
5.   Reproduce the recombinant
     bacteria.
6.   The foreign genes will be expressed
     in the bacteria.
1.   It must be able to replicate
2.   There must be some way to introduce
     vector DNA into the cell
3.   There must be some way of detecting its
     presence, preferably by plating techniques

Most common vectors are:
 Plasmid, phage λ and viruses
   Discovered in an experiment where
    bacteriophage lost its plaque formation in
    E.coli
   Enzymes that recognize a specific base
    sequence in a DNA molecule
   It makes two cuts, one in each strand,
    generating 3’-OH and 5’-P termini
   Types of termini produced:
     Flush or blunt end
     Cohesive or sticky end
   The number of cuts made in the DNA from
    specific organism is limited
   A particular restriction enzyme generates a
    unique family fragments from a DNA
    molecule
•BstEII pUC19 pUC19 •HindIII   •HindIII   •BstEII
Restriction maps show the relative location of a selection of restriction sites along
        linear or circular DNA.


              EcoRI
                       HindIII

PstII                     BamHI
                                      HindIII   BamHI                         PstII
Digests
1: EcoRI
2: HindIII
3: EcoRI + HindIII
Resultant Fragments: approximate sizes
1: 3 kb, 5 kb
2: 6 kb, 2 kb
3: 2 kb, 1 kb, 5 kb,
BglII            BglII             BamHI
BglII                BamHI         PstI           +BamHI           +PstI             +PstI


                             5.2
              4.2
                                            3.6            3.5
                                                                            3.3
                                                                                             2.6

              1.7                                          1.7
                                            1.4                                              1.4
                                            1.2                            1.2               1.2
                             1.0                                           0.9               1.0
                                                           0.7
                                                                           0.5
              0.3                                          0.3             0.3


      BglII          BamHI                                 PstI         BglII PstI

0.3            0.7                    2.6                         0.9      0.5         1.2
A) 11, 6, 5
B) 14,8
C) 16,6

A x B) 8, 6, 5, 3
A x C) 11, 5, 5, 1
B x C) 8, 8, 6
   Cohesive end
   Blunt end
     Increasing the DNA concentration and addition of
      ligase
     Addition of homopolymers
     Using of linkers
   Antibiotic resistance marker
     Insertional inactivation
   Electrophoresis
   hybridization
   collection of all of the vector molecules, each
    carrying a piece of the chromosomal DNA of
    the organism
Microbial genetics and genetic engineering

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Microbial genetics and genetic engineering

  • 2. Mutagen Gene transfer Genetic recombi nation Selection of mutants
  • 4. Genetic engineering involves changing the genetic material in an organism to alter its traits or products • A recombinant DNA molecule contains DNA fragments spliced together from 2 or more organisms
  • 5. Stages of cloning experiment  Elements:  Vectors  Restriction enzymes  Mechanism in joining the fragments  Selection or detection of successful cloning  Gene library
  • 6. 1. Joining DNA segment Vector 2. Providing milieu that allows propagation Clones
  • 7. 1. Remove bacterial DNA (plasmid). 2. Cut the Bacterial DNA with “restriction enzymes”. 3. Cut the DNA from another organism with “restriction enzymes”. 4. Combine the cut pieces of DNA together with another enzyme and insert them into bacteria. 5. Reproduce the recombinant bacteria. 6. The foreign genes will be expressed in the bacteria.
  • 8. 1. It must be able to replicate 2. There must be some way to introduce vector DNA into the cell 3. There must be some way of detecting its presence, preferably by plating techniques Most common vectors are:  Plasmid, phage λ and viruses
  • 9. Discovered in an experiment where bacteriophage lost its plaque formation in E.coli  Enzymes that recognize a specific base sequence in a DNA molecule  It makes two cuts, one in each strand, generating 3’-OH and 5’-P termini  Types of termini produced:  Flush or blunt end  Cohesive or sticky end
  • 10.
  • 11.
  • 12. The number of cuts made in the DNA from specific organism is limited  A particular restriction enzyme generates a unique family fragments from a DNA molecule
  • 13. •BstEII pUC19 pUC19 •HindIII •HindIII •BstEII
  • 14. Restriction maps show the relative location of a selection of restriction sites along linear or circular DNA. EcoRI HindIII PstII BamHI HindIII BamHI PstII
  • 15. Digests 1: EcoRI 2: HindIII 3: EcoRI + HindIII Resultant Fragments: approximate sizes 1: 3 kb, 5 kb 2: 6 kb, 2 kb 3: 2 kb, 1 kb, 5 kb,
  • 16. BglII BglII BamHI BglII BamHI PstI +BamHI +PstI +PstI 5.2 4.2 3.6 3.5 3.3 2.6 1.7 1.7 1.4 1.4 1.2 1.2 1.2 1.0 0.9 1.0 0.7 0.5 0.3 0.3 0.3 BglII BamHI PstI BglII PstI 0.3 0.7 2.6 0.9 0.5 1.2
  • 17. A) 11, 6, 5 B) 14,8 C) 16,6 A x B) 8, 6, 5, 3 A x C) 11, 5, 5, 1 B x C) 8, 8, 6
  • 18. Cohesive end  Blunt end  Increasing the DNA concentration and addition of ligase  Addition of homopolymers  Using of linkers
  • 19.
  • 20.
  • 21.
  • 22. Antibiotic resistance marker  Insertional inactivation  Electrophoresis  hybridization
  • 23.
  • 24.
  • 25. collection of all of the vector molecules, each carrying a piece of the chromosomal DNA of the organism

Notes de l'éditeur

  1. This events could be so complex when using natural and random mutagens and then selection. That is why scientists develop technology that can modify organism in directed and predetermined way
  2. RE are enzymes that can cut
  3. Restriction mapping??