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Enzymes and proteins in DNA
        replication




               Presented by
               R.Parthasarathy
Introduction
• Multiple proteins are required for DNA
  replication at a replication fork.
• These include DNA polymerases, single-strand
  DNA binding proteins, helicases,
  primase,topoisomerases, and DNA ligase.
  Some of these are multisubunit protein
  complexes.
dnaA Protein
• The base sequence at the origin of replication
  is recognized and bound by the dna A protein.
Helicase
• Helicase uses energy from the ATP to break the
  hydrogen bonds holding the base pairs together.
• This allows the two parental strands of DNA to
  begin unwinding and forms two replication
  forks.
• Each strand of parental DNA has it own helicase.
• In humans, two inherited diseases, Werner's
  syndrome and Bloom's syndrome, result from
  helicase defects.
• E. coli contains at least 6 different helicases--
  some involved in DNA repair and others in
  conjugation, the principal helicase in DNA
  replication is DnaB
SSB Protein
• Single-stranded DNA binding protein (SSB) binds to the
  single-stranded portion of each DNA strand, preventing the
  strands from reassociating and protecting them from
  degradation by nucleases.
• gp32, the most studied SSB protein, binds in a strongly
  cooperative fashion to single-strand DNA.
• That is, binding adjacent to another gp32 is much more likely
  than the binding of a single gp32 in isolation.
• This property helps promote the denaturation of duplex DNA and
  helps keep the DNA template in an extended, single-strand
  conformation, with the purine and pyrimidine bases exposed so
  that they can base-pair readily with incoming nucleotides.
• In E. coli, the protein is called ssb.
• In eukaryotic cells, a heterotrimeric protein called replication
  factor A serves the role of SSB in DNA replication.
Primase
• Primase is an enzyme that copies a DNA template
  strand by making an RNA strand complementary to it.
• Primase synthesizes a short (about 10 nucleotides)
  RNA primer in the 5’ 3’ direction.
• The parental strand is used as a template for this
  process.
• RNA primers are required because DNA polymerases
  are unable to initiate synthesis of DNA, but can only
  extend a strand from the 3' end of a preformed
  “primer”
• The enzyme is active only in the presence of other
  proteins (including a helicase), which create a complex
  called the primosome
DNA polymerase III
• It catalyzes the chemical reactions for
  polymerization of nucleotides.
• DNA polymerase III begins synthesizing DNA
  in the 5’ 3’direction, beginning at the 3’
  end of each RNA primer.
• The newly synthesized strand is
  complementary and antiparallel to the
  parental strand used as a template.
DNA polymerase I
• DNA polymerase I and RNAse H are involved in removing RNA
  primers in the processing of DNA after replication.
• This enzyme removes the ribonucleotides one at a time
  from the 5' end of the primer (5‘ 3' exonuclease).
• DNA polymerase I also fills in the resulting gaps by
  synthesizing DNA, beginning at the 3' end of the
  neighbouring Okazaki fragment.
• Both DNA polymerase I and III have the ability to
  "proofread" their work by means of a 3' 5' exonuclease
   activity.
• If DNA polymerase makes a mistake during DNA synthesis,
  the resulting unpaired base at the 3' end of the growing
    strand is removed before synthesis continues.
Comparison of DNA and RNA
polymerases
                            DNA Polymerase           RNA Polymerase

 Nucleic acid synthesized   DNA                      RNA
 (5’  3’)


 Required template          DNA*                     DNA*

 Required substrates        dATP, dGTP, dCTP, dTTP   ATP, GTP, CTP, UTP

 Required primer            RNA (or DNA)             None

 Proofreading activity      Yes                      No
 (3’  5’ exonuclease)
Clamps and clamp loaders
• Protein from the DNA polymerase III
  holoenzyme
   complex holds the polymerase to the DNA.
• This helps the DNA polymerase complex to
  stay on the DNA through an entire cycle of
  replication.
• A multi subunit entity called the complex
  functions as the "clamp loader". That is, it
  loads the clamp onto the DNA.
Clamps and clamp loaders
• a protein dimer that encircles the DNA strand
  and helps hold the DNA polymerase to the
  DNA strand.
• In eukaryotic cells, a multi-subunit protein
  called replication factor C (RF-C) is the clamp
  loader, and proliferating cell nuclear antigen
  (PCNA) is the sliding clamp.
DNA ligase
• DNA ligase seals the "nicks" between
  Okazaki fragments, converting them to a
  continuous strand of DNA.
• Covalently closes nicks in double-stranded
  DNA.
DNA gyrase
• DNA gyrase (DNA topoisomerase II) provides a
  "swivel" in front of each replication fork.
• As helicase unwinds the DNA at the replication
  forks, the DNA ahead of it becomes overwound and
   positive supercoils form.
• DNA gyrase inserts negative supercoils by nicking
  both strands of DNA, passing the DNA strands
  through the nick, and then resealing both strands
  again.
• DNA topoisomerase I can relieve supercoiling in DNA
  molecules by the transient breaking and resealing of
  just one of the strands of DNA.
Action of a gyrase
Action of a type I topoisomerase
Step in Replication             Prokaryotic cells              Eukaryotic cells

Recognition of origin of                Dna A protein                   Unknown
replication
Unwinding of DNA double helix              Helicase                      Helicase
                                        (requires ATP)                (requires ATP)
Stabilization of unwound         Single-stranded DNA-binding   Single-stranded DNA-binding
template strands                          protein (SSB)                 protein (SSB)
Synthesis of RNA primers                   Primase                       Primase
Synthesis of DNA
Leading strand                       DNA polymerase III            DNA polymerase δ
Lagging strand                       DNA polymerase III            DNA polymerase α
Removal of RNA primers               DNA polymerase I                   Unknown
                                   (5 3' exonuclease)
Replacement of RNA with DNA          DNA polymerase I                   Unknown

Joining of Okazaki fragments              DNA ligase                   DNA ligase
                                       (requires NAD)                (requires ATP)
Removal of positive supercoils      DNA topoisomerase II          DNA topoisomerase II
ahead of advancing                     (DNA gyrase)
replication forks
References
MOLECULAR BIOLOGY by David Clark
Genes VII

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Enzymes and proteins in dna replication

  • 1. Enzymes and proteins in DNA replication Presented by R.Parthasarathy
  • 2. Introduction • Multiple proteins are required for DNA replication at a replication fork. • These include DNA polymerases, single-strand DNA binding proteins, helicases, primase,topoisomerases, and DNA ligase. Some of these are multisubunit protein complexes.
  • 3. dnaA Protein • The base sequence at the origin of replication is recognized and bound by the dna A protein.
  • 4. Helicase • Helicase uses energy from the ATP to break the hydrogen bonds holding the base pairs together. • This allows the two parental strands of DNA to begin unwinding and forms two replication forks. • Each strand of parental DNA has it own helicase. • In humans, two inherited diseases, Werner's syndrome and Bloom's syndrome, result from helicase defects. • E. coli contains at least 6 different helicases-- some involved in DNA repair and others in conjugation, the principal helicase in DNA replication is DnaB
  • 5. SSB Protein • Single-stranded DNA binding protein (SSB) binds to the single-stranded portion of each DNA strand, preventing the strands from reassociating and protecting them from degradation by nucleases. • gp32, the most studied SSB protein, binds in a strongly cooperative fashion to single-strand DNA. • That is, binding adjacent to another gp32 is much more likely than the binding of a single gp32 in isolation. • This property helps promote the denaturation of duplex DNA and helps keep the DNA template in an extended, single-strand conformation, with the purine and pyrimidine bases exposed so that they can base-pair readily with incoming nucleotides. • In E. coli, the protein is called ssb. • In eukaryotic cells, a heterotrimeric protein called replication factor A serves the role of SSB in DNA replication.
  • 6. Primase • Primase is an enzyme that copies a DNA template strand by making an RNA strand complementary to it. • Primase synthesizes a short (about 10 nucleotides) RNA primer in the 5’ 3’ direction. • The parental strand is used as a template for this process. • RNA primers are required because DNA polymerases are unable to initiate synthesis of DNA, but can only extend a strand from the 3' end of a preformed “primer” • The enzyme is active only in the presence of other proteins (including a helicase), which create a complex called the primosome
  • 7. DNA polymerase III • It catalyzes the chemical reactions for polymerization of nucleotides. • DNA polymerase III begins synthesizing DNA in the 5’ 3’direction, beginning at the 3’ end of each RNA primer. • The newly synthesized strand is complementary and antiparallel to the parental strand used as a template.
  • 8. DNA polymerase I • DNA polymerase I and RNAse H are involved in removing RNA primers in the processing of DNA after replication. • This enzyme removes the ribonucleotides one at a time from the 5' end of the primer (5‘ 3' exonuclease). • DNA polymerase I also fills in the resulting gaps by synthesizing DNA, beginning at the 3' end of the neighbouring Okazaki fragment. • Both DNA polymerase I and III have the ability to "proofread" their work by means of a 3' 5' exonuclease activity. • If DNA polymerase makes a mistake during DNA synthesis, the resulting unpaired base at the 3' end of the growing strand is removed before synthesis continues.
  • 9. Comparison of DNA and RNA polymerases DNA Polymerase RNA Polymerase Nucleic acid synthesized DNA RNA (5’  3’) Required template DNA* DNA* Required substrates dATP, dGTP, dCTP, dTTP ATP, GTP, CTP, UTP Required primer RNA (or DNA) None Proofreading activity Yes No (3’  5’ exonuclease)
  • 10. Clamps and clamp loaders • Protein from the DNA polymerase III holoenzyme complex holds the polymerase to the DNA. • This helps the DNA polymerase complex to stay on the DNA through an entire cycle of replication. • A multi subunit entity called the complex functions as the "clamp loader". That is, it loads the clamp onto the DNA.
  • 11. Clamps and clamp loaders • a protein dimer that encircles the DNA strand and helps hold the DNA polymerase to the DNA strand. • In eukaryotic cells, a multi-subunit protein called replication factor C (RF-C) is the clamp loader, and proliferating cell nuclear antigen (PCNA) is the sliding clamp.
  • 12. DNA ligase • DNA ligase seals the "nicks" between Okazaki fragments, converting them to a continuous strand of DNA. • Covalently closes nicks in double-stranded DNA.
  • 13. DNA gyrase • DNA gyrase (DNA topoisomerase II) provides a "swivel" in front of each replication fork. • As helicase unwinds the DNA at the replication forks, the DNA ahead of it becomes overwound and positive supercoils form. • DNA gyrase inserts negative supercoils by nicking both strands of DNA, passing the DNA strands through the nick, and then resealing both strands again. • DNA topoisomerase I can relieve supercoiling in DNA molecules by the transient breaking and resealing of just one of the strands of DNA.
  • 14. Action of a gyrase
  • 15. Action of a type I topoisomerase
  • 16.
  • 17. Step in Replication Prokaryotic cells Eukaryotic cells Recognition of origin of Dna A protein Unknown replication Unwinding of DNA double helix Helicase Helicase (requires ATP) (requires ATP) Stabilization of unwound Single-stranded DNA-binding Single-stranded DNA-binding template strands protein (SSB) protein (SSB) Synthesis of RNA primers Primase Primase Synthesis of DNA Leading strand DNA polymerase III DNA polymerase δ Lagging strand DNA polymerase III DNA polymerase α Removal of RNA primers DNA polymerase I Unknown (5 3' exonuclease) Replacement of RNA with DNA DNA polymerase I Unknown Joining of Okazaki fragments DNA ligase DNA ligase (requires NAD) (requires ATP) Removal of positive supercoils DNA topoisomerase II DNA topoisomerase II ahead of advancing (DNA gyrase) replication forks
  • 18. References MOLECULAR BIOLOGY by David Clark Genes VII