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DNA Sequencing
Genetic Engineering
• Problem – getting enough raw
  material
  – Old solution: “bucket biochemistry”
  – New solution: Polymerase Chain
    Reaction
PCR
• PCR is the cloning of DNA (amplification).
• Copies are made and the amount of DNA
  can be rapidly increased. Useful if the
  source of DNA is small.
• Temperature is used instead of enzymes
  like helicases (95oC ).
• DNA polymerase is thermostable to
  protect it against the reaction
  temperatures.
• This is an automated process and can
  produce sufficient DNA in 20 cycles.
PCR
PCR
DNA Sequencing
• Concept: If we know the distance of each type of base from
  a known origin,
  then it is possible to deduce the sequence of the DNA.

• For example, if we knew that there was an:

•   A at positions 2, 3, 11, 13 ... and
•   G at positions 1, 12, ... and
•   C at positions 6, 7, 8, 10, 15... and
•   T at positions 4, 5, 9, 14....

• then we can reconstruct the sequence
DNA Sequencing
• Obtaining this information is conceptually quite
  simple. The idea is to cause a termination of a
  growing DNA chain at a known base (A,G,C or T)
  and at a known location in the DNA

• In practice, chain termination is caused by the
  inclusion of a small amount of a single
  dideoxynucleotide base in the mixture of all four
  normal bases (e.g. dATP, dTTP, dCTP, dGTP and
  ddATP). The small amount of ddATP would cause
  chain termination whenever it would be
  incorporated into the DNA. The incorporation of
  ddATP would be random and thus all possible
  chains that end in 'A' will exist.
DNA Sequencing
DNA Sequencing
DNA Sequencing



The separation of the sequencing fragments
DNA Sequencing



Snapshots of the
detection of the
fragments on the
sequencer




                   four-dye system   single-dye system
Gel Electrophoresis
• DNA is “cut” with a restriction enzyme
• Sample of fragmented DNA is placed in
  one of the wells on the gel.
• An electrical current is passed across the
  gel.
• Fragment separation is based on charge
  and size.
• Large fragments move slowly.
• Negative fragments are moved to the
  right.
Gel Electrophoresis
Gel Electrophoresis
• This diagram shows the
  separation of 6 separate
  mixtures of DNA.
• The dark bands to the left
  are those with a large
  molecular mass or a
  positive charge
• The top mixture contains 5
  fragments of DNA. Each
  bands corresponds to a
  group of DNA molecules of
  the same size and charge.
• The 2nd and 5th samples
  have the same bands.


                               -
  They are identical.

                                   +
DNA Profiling
• The technique can be used in:
• Forensic crime investigations
• Parentage Issues
• Animal breeding pedigrees
• Disease detection
Fingerprinting

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Dna sequencing

  • 2. Genetic Engineering • Problem – getting enough raw material – Old solution: “bucket biochemistry” – New solution: Polymerase Chain Reaction
  • 3. PCR • PCR is the cloning of DNA (amplification). • Copies are made and the amount of DNA can be rapidly increased. Useful if the source of DNA is small. • Temperature is used instead of enzymes like helicases (95oC ). • DNA polymerase is thermostable to protect it against the reaction temperatures. • This is an automated process and can produce sufficient DNA in 20 cycles.
  • 4. PCR
  • 5. PCR
  • 6. DNA Sequencing • Concept: If we know the distance of each type of base from a known origin, then it is possible to deduce the sequence of the DNA. • For example, if we knew that there was an: • A at positions 2, 3, 11, 13 ... and • G at positions 1, 12, ... and • C at positions 6, 7, 8, 10, 15... and • T at positions 4, 5, 9, 14.... • then we can reconstruct the sequence
  • 7. DNA Sequencing • Obtaining this information is conceptually quite simple. The idea is to cause a termination of a growing DNA chain at a known base (A,G,C or T) and at a known location in the DNA • In practice, chain termination is caused by the inclusion of a small amount of a single dideoxynucleotide base in the mixture of all four normal bases (e.g. dATP, dTTP, dCTP, dGTP and ddATP). The small amount of ddATP would cause chain termination whenever it would be incorporated into the DNA. The incorporation of ddATP would be random and thus all possible chains that end in 'A' will exist.
  • 8.
  • 9.
  • 12. DNA Sequencing The separation of the sequencing fragments
  • 13. DNA Sequencing Snapshots of the detection of the fragments on the sequencer four-dye system single-dye system
  • 14. Gel Electrophoresis • DNA is “cut” with a restriction enzyme • Sample of fragmented DNA is placed in one of the wells on the gel. • An electrical current is passed across the gel. • Fragment separation is based on charge and size. • Large fragments move slowly. • Negative fragments are moved to the right.
  • 16. Gel Electrophoresis • This diagram shows the separation of 6 separate mixtures of DNA. • The dark bands to the left are those with a large molecular mass or a positive charge • The top mixture contains 5 fragments of DNA. Each bands corresponds to a group of DNA molecules of the same size and charge. • The 2nd and 5th samples have the same bands. - They are identical. +
  • 17. DNA Profiling • The technique can be used in: • Forensic crime investigations • Parentage Issues • Animal breeding pedigrees • Disease detection

Notas do Editor

  1. DNA/RNA overview
  2. DNA/RNA overview
  3. DNA/RNA overview