2.7 + 7.1 Replication Flashcards

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1
Q

Why is DNA replication semi-conservative?

A

Semi-conservative:

  • in new helix one strand is from template
  • another strand is newly synthesised
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2
Q

Steps of DNA replication + enzymes

A
  1. Uncoils double strand, breaks H bonds - helicase (uses ATP) and DNA gyrase (topoisomerase)- replication fork created
  2. Single stranded binding proteins attach - prevent strands from pairing
  3. DNA polymerase III (always 5’->3’) attaches to leading strand and continuously synthesises new strand 5’ to 3’ end (free nucleotides)
  4. DNA (RNA) primase adds RNA primer to lagging strand - DNA polymerase III synthesises in Okazaki fragments

5. DNA polymerase I removes primers - DNA ligase seals fragments

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3
Q

Evidence for semi-conservative DNA replication

A

Meselson-Stahl experiment

  • 15N - radioactive isotope in medium - bacteria cultured
  • almost all N were radioactive
  • transferred bacteria to 14N medium - after some time samples of DNA collected
  • DNA density measured by centrifugation with CsCl
  • after 2 generations there were no DNA strands with only 15N

= this pattern can only be seen if replication is semi-conservative

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4
Q

DNA helicase structure

A

From six globular proteins - donut shape

Uses ATP to break H bonds between complementary bases

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5
Q

DNA polymerase

A
  • brings nucleotides into the position where they can form H bonds
  • links the nucleotide to the strand by covalent bonds between free nucleotide phosphate and strang sugar
  • pentose is 3’ end, phosphate 5’ end
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6
Q

PCR process

A

Components:

  • Taq polymerase (heat resistant from themophilic bacteria)
  • primers
  • free nucleotides
  • DNA sample
  • buffer

Process:

  • Denaturing: strands separate
  • Annealing: primers bind
  • Elongation: syntehsis of new strand
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7
Q

Enzymes involved in DNA replication

A
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8
Q

How DNA sequencing is completed?

A

Sanger method

  • Different fluorescent dyes attached to ndideoxynucleotides (after they attached - strand no longer elongated)
  • Length of fragment (electropohoresis) determines position of that nucleotide (A, C, G, T)
    1. Four free nucleotide mixes prepared - many normal + one ddA/ddC/ddG/ddT
    4. PCR
    5. Gel electrophoresis
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9
Q

Types of non-coding DNA

A
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10
Q

DNA profiling technique

A
  • uses: paternity tests, forensic investigations
  • introns unique in each individual - satellite DNA - short tandem repeats

Procedure:

  1. DNA sample
  2. PCR
  3. Electrophoresis
  4. Comparison of STR bands
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11
Q

Eukaryotic DNA packing

A
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12
Q

Nucleosome structure

A
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