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Molecular Biology Techniques

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Harpers Biochemistry (23rd ed.) Murray et al. 42. Instant Notes in Biochem. ( 1997) ... Biochemistry (Mols., Cells and the Body) Dow et al. Lippincotts Illus. ... – PowerPoint PPT presentation

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Title: Molecular Biology Techniques


1
Molecular Biology Techniques
2
Why Use Molecular Biology Techniques?
  • Gene mutations can have serious consequences
  • Dental diseases include amelogenesis and
    dentinogenesis imperfecta
  • Also more severe diseases such as cystic fibrosis
  • Molecular biology techniques can help to
    differentiate between normal genes and mutations

3
Human Genome Project
  • Elucidation of genes will allow for development
    of accurate diagnostics for treatment of diseases
  • Single genes associated with cystic fibrosis and
    muscular dystrophy found
  • Also discovery of diseases caused by several
    genes/gene interacting with environment

4
Aims Objectives
  • To examine the method and application of
  • Restriction endonucleases
  • Gene cloning and expression using plasmid cloning
    vectors
  • Polymerase Chain Reaction
  • Southern Blotting and nucleic acid hybridisation
  • DNA sequencing

5
Restriction Endonucleases
  • Important tools in recombinant technology
  • Have opened the way for gene cloning
  • Endonucleases provide protection to bacterial
    cell against foreign DNA
  • Bacterias own DNA is modified by methylation of
    bases

6
  • Enzymes are named from bacterial species that
    they are derived from
  • EcoRI ? is the first enzyme to be isolated from
    E. coli strain RY13
  • The enzymes recognise 4-6bp of DNA and cleave
    phosphodiester bond

7
  • Restriction site is palindrome ?
  • EcoRI
  • forward 5-3 GAATTC
  • reverse 3-5 CTTAAG
  • Digestion with EcoRI gives staggered end other
    enzymes produce blunt ends ?
  • EcoRI HaeIII
  • G AATTC GG CC
  • CTTAA G CC GG

8
  • Restricted fragments can be separated by size
    using gel electrophoresis
  • Standard markers run alongside used to size them
  • Polyacrylamide gels used to separate low
    molecular weight molecules
  • Agarose gels used to separate out high molecular
    weight molecules

9
Plasmids and Gene Cloning
  • Extrachromosomal DNA molecules
  • Confer antibiotic resistance
  • Vectors are plasmids designed for gene cloning
  • 3 basic requirements of vectors
  • ability to self replicate within host
  • possession of selection marker
  • must be capable of being digested

10
  • When vector and DNA are digested with the same
    enzymes both can be joined together using DNA
    ligase
  • DNA ligase catalyses formation of phosphodiester
    bond
  • Resulting recombinant DNA can be introduced into
    cells treated to make them permeable

11
  • As cells divide and grow, recombinant plasmid
    replicates many times
  • Relevant clones can be selected by use of
    antibiotic within media
  • Only DNA lt10kb can be inserted into vectors

12
Polymerase Chain Reaction
  • Amplifies DNA molecules exponentially using DNA
    polymerase
  • Only flanking sequence of DNA needs to be known
    for design of primers
  • Primers are short oligonucleotides (20-35)
    representing forward and reverse sequences
  • Each primer anneals to 3 portion of the DNA
    template

13
Recommended Reading
  • Biochemistry (2002) Stryer
    6
  • Biochemistry (1995) Voet and Voet
    28
  • Mol. Cell Biology (2000) Lodish et al.
    7
  • Mol. Biology of the Cell (2002) Alberts et al.
    7
  • Harpers Biochemistry (23rd ed.) Murray et al.
    42
  • Instant Notes in Biochem. (1997) Hames et
    al. I
  • Instant Notes in Mol. Biol. (1997) Turner et al.
    G/H/I/J
  • Biochemistry (Mols., Cells and the Body) Dow
    et al. -
  • Lippincotts Illus. Reviews (2nd ed.) Champe and
    Harvey 33

14
Aims Objectives
  • To examine the method and application of
  • Restriction endonucleases
  • Gene cloning and expression using plasmid
    cloning vectors
  • Polymerase Chain Reaction
  • Southern Blotting and nucleic acid hybridisation
  • DNA sequencing

15
Southern Blotting
  • Used to detect copy number of gene
  • Can also detect gross alterations in a gene
  • Allows for visualisation of specific DNA fragment
    among thousands of molecules
  • Can probe for more than one fragment of DNA

16
Southern Blot Procedure
  • Digested DNA with appropriate restriction enzyme
  • Run fragments on electrophoresis gel to separate
  • Denature DNA to make single strands and transfer
    to nitrocellulose membrane
  • Hybridise DNA with specific probe
  • Detect DNA fragment

17
Hybridisation of Nucleic Acids
  • Heating causes DNA to denature into single
    strands they can re-anneal when temperature
    lowered
  • For annealing to occur require sufficient
    complementary nucleotide sequence between the two
    nucleic acid molecules
  • Annealing can be achieved with any two single
    stranded nucleic acid molecules

18
  • Hybridisation can be used to establish success of
    cloning experiment
  • For RNA it can be used as an indication of the
    level of gene expression
  • Specific probe can be DNA fragment, cloned DNA or
    synthetic oligonucleotide
  • Labelling of probe is usually with 32P
  • Same basic method for all forms of nucleic acids

19
DNA Sequencing
  • Sanger technique used frequently these days
  • Uses dideoxynucleotides to terminate chain
    elongation during DNA synthesis
  • Radioactive nucleotide incorporated into
    elongating strands
  • Four reactions carried out simultaneously,
    containing 4dNTPs and single ddNTP

20
Extension of Polynucleotide Chain
21
  • Extension reaction products are resolved by gel
    electrophoresis
  • Results obtained when gel is dried and exposed to
    X-ray film
  • Bands near bottom of gel represent short reaction
    products those at top the longest
  • The process is now automated and uses fluorescent
    dye

22
Sanger Technique for Sequencing
23
Recommended Reading
  • Biochemistry (2002) Stryer
    6
  • Biochemistry (1995) Voet and Voet
    28
  • Mol. Cell Biology (2000) Lodish et al.
    7
  • Mol. Biology of the Cell (2002) Alberts et al.
    7
  • Harpers Biochemistry (23RD Ed.) Murray et al.
    42
  • Instant Notes in Biochem. (1997) Hames et
    al. I
  • Instant Notes in Mol. Biol. (1997) Turner et al.
    G/H/I/J
  • Biochemistry (Mols., Cells and the Body) Dow
    et al. -
  • Lippincotts Illus. Reviews (2nd Ed.) Champe and
    Harvey 33
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