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HEENA KAUSAR
Govt. E. Raghvendra Rao PG
Science College
 All organisms must duplicate their DNA with
extraordinary accuracy before each cell division.
 DNA replication is a biological process that occurs in
all living organisms and copies their exact DNA. It is
the basis for biological inheritance.
 Replication is the process of synthesis of daughter
DNA from parental DNA by the enzyme DNA
Polymerase.
 DNA templating is the process in which the nucleotide
sequence of a DNA strand (or selected portions of a
DNA strand) is copied by complementary base-pairing
(A with T, and G with C) into a complementary DNA
sequence.
DNA RNA PROTEIN
Transcription Translation
Replication
Reverse
transcription
Parental strand
Daughter stand
⚫A reaction in which daughter DNAs are
synthesized using the parental DNAs as
the template.
⚫Transferring the genetic information to
the descendant generation with a high
fidelity.
Replication
Parental DNA
Daughter DNA
6
1. Semiconservative replication
2. Conservative replication
3. Dispersive replication
Conservative
replication
Dispersive
replication
Semiconservative replication
Parentstrands
New / Daughter
strand
 Semi-conservative replication
 Bidirectional replication
 Semi-continuous replication
 High fidelity
10
Cells broken open
to extract DNA
E. coli grown in the presence
of 15N (a heavy isotope of
Nitrogen) for many generations
only 14N (a light
isotope of Nitrogen)
Sampled
at:
0 min
1
• Cells get heavy-labeled DNA
2
E. coli placed in
medium containing
3
40
min
20
min
Suspended DNA in Cesium
chloride (CsCl) solution.
4
15N medium
CsCl density gradient
centrifugation
5
15N
14N
DNA
Both
strands
heavy
F1
generation
DNA (one
heavy/one
light strand)
0 min 20 min 40 min
F2 generation
DNA:
 Two light
strands
 One heavy/One
light strand
Three
rounds of
replication:
Original
DNA
1st Round:
2nd
Round:
3rd
Round:
0 min
20 min
40 min
60
min?
Identical
base sequences
3’ 5’
5’
3’
3’
Half of the parental DNA molecule
is conserved in each new double helix,
paired with a newly synthesized
complementary strand. This is called
semiconservative replication.
• Replication starts from unwinding the
dsDNA at a particular point (called
origin / ori site), followed by the
synthesis on each strand.
• The parental dsDNA and two newly
formed dsDNA form a Y-shape
structure called Replication fork.
The replication
process starts
from the origin,
and proceeds in
two opposite
directions.
It is named
- Replication.
21
• DNA Polymerase - Matches the
correct nucleotides then joins /
polymerizes adjacent nucleotides to
each other.
• Helicase - Unwinds the DNA and
melts it.
• Primase - Provides an RNA primer to
start polymerization.
• Single Strand Binding Proteins - Keep
the DNA single stranded after it has been
melted by helicase
• Gyrase - A topisomerase that Relieves
torsional strain in the DNAmolecule.
• Ligase - Joins adjacent DNA strands
together (fixes “nicks”)
• Telomerase - Finishes off the ends of DNA
strands in Eukaryotes
DNA Polymerase-I
• The first DNA- dependent DNA
polymerase ( DNA Pol -I ) was
discovered in 1958 by Arthur
Kornberg who received Nobel
Prize in physiology & medicine
in 1959.
• DNA Polymerase is considered
as Kornberg Enzyme.
• Later, DNA-Pol II and DNA-Pol
III were identified.
• All of them possess the
following biological activity.
• 53 Polymerse activity
• Exonuclease activity
3´→5´ exonuclease
activity
excise mismatched
nuleotides
A G G A
A A G T C C G G C G
5´→3´
exonuclease
activity
removes primer or
excise mutated
segment
5'
C T T C
3'
3'
G
5'
⚫Mainly responsible
for proofreading and
filling the gaps,
repairing DNA
damage
30
• Small fragment (323 AA): having
5´→3´ exonuclease activity
• Large fragment (604 AA): called Klenow
fragment, having DNA polymerization
and 3´→5´exonuclease activity
Large fragment
Small fragment
C-end
DNA-pol
Ⅰ Cleavage
• Temporarily functional when DNA-pol
I and DNA-pol III are not functional.
• Still capable for doing synthesis on
the damaged template.
• Participates in DNArepair process.
• A heterodimer enzyme composed
of ten different subunits
• Having the highest
polymerization activity (105
nt/min)
• The true enzyme responsible for
the elongation process
α: has 5´→ 3´
polymerizing activity
ε:has 3´→ 5´
exonuclease activity and
plays a key role to ensure
the replication fidelity.
θ: maintain heterodimer
structure
Free 3’- hydroxyl group
• Also called DnaG
• Primase is able to synthesize primers
using free NTPs as the substrate and
the ssDNAas the template.
• Primers are short RNA fragments of a
several nucleotides long.
• Primers provide free 3´-OH groups to
react with the -P atom of dNTP to
form phosphodiester bonds.
• Primase, DnaB, DnaC and an origin
form a Primosome complex at the
initiation phase.
• Also referred to as DnaB.
• It opens the double strand DNAwith
consumingATP.
• The opening process with the assistance
of DnaAand DnaC
• Single Strand DNABinding protein.
• SSB protein maintains the DNA
template in the single strand form in
order to
• prevent the dsDNAformation;
• protect the vulnerable ssDNA from
nucleases.
• It cuts phosphoester bonds on both
strands of dsDNA, releases the
supercoil constraint, and reforms the
phosphodiester bonds.
• It can change dsDNA into the negative
supercoil state with consumption of
ATP.
3'
5'
5'
3'
RNAase
P
OH
3'
5'
5'
3'
DNA polymerase
P
3'
5'
5'
3'
dNTP
DNAligase
3'
5'
5'
3'
ATP
• Connect two adjacent ssDNA strands
by joining the 3´-OH of one DNA
strand to the 5´-P of another DNA
strand.
• Sealing the nick in the process of
Replication, Repairing, Recombination,
and Splicing.
• Replication based on the principle of
base pairing is crucial to the high
accuracy of the genetic information
transfer.
• Enzymes use two mechanisms to
ensure the replication fidelity.
–Proofreading and real-time correction
–Base selection
• DNA-pol I has the function to correct
the mismatched nucleotides.
• It identifies the mismatched nucleotide,
removes it using the 3´- 5´ exonuclease
activity, add a correct base, and
continues the replication.
DNA REPLICATION
Initiation
Elongation
Termination
1) Initiation
• Occurs at the origin of replication
• Separates dsDNA, primer synthesis
2) Elongation
• Involves the addition of new nucleotides (dNTPs )
based on complementarity of the template strand
• Forms phosphoester bonds, correct the mismatch bases,
extending the DNAstrand, …
3) Termination
• Stops the DNAReplication occurs at a specific
termination site
• The replication starts at a particular point
called origin of Replication (or) ori-Site.
• The structure of the origin is 248 bp long andAT-rich.
9 mer- sequence
13 mer- sequence
Site where DNA synthesis
starts
• DnaArecognizes ori C.
• DnaB ( Helicase ) and DnaC join the DNA-
DnaA complex, open the local AT-rich
region, and move on the template
downstream further to separate enough
space.
• DnaAis replaced gradually.
• SSB protein binds the complex to
stabilize ssDNA.
• Primase joins and forms a complex
called primosome.
• Primase starts the synthesis of primers
on the ssDNA template using NTP as the
substrates in the 5´- 3´ direction at the
expense ofATP.
• The short RNA fragments provide
free 3´-OH groups for DNA
elongation.
Primase synthesizes PRIMER
’
Single stranded binding protein
Initiation
⚫dNTPs are continuously connected to the
primer or the nascent DNA chain by
DNA-pol III.
⚫The core enzymes (、、and  ) catalyze
the synthesis of leading and lagging
strands, respectively.
⚫The nature of the chain elongation is the
series formation of the phosphodiester
bonds.
3’
3’ Laging strand
5’
Okazaki fragments
Gap filled byDNA Ligase
Pri
E
m
lo
en
rg
is
at
rie
om
no
bv
y
eD
dNb
A
yP
D
oN
lyA
mP
er
oa
ly
se
m
Ie
II
rase I
• RNA Primers on Okazaki fragments
are digested by the enzyme RNase.
• The gaps are filled by DNA-pol I in
the 5´→3´direction.
• The nick between the 5´end of one
fragment and the 3´end of the next
fragment is sealed by ligase.
• Many DNA fragments are synthesized
sequentially on the DNA template strand
having the 5´- end. These DNA fragments
are called Okazaki fragments.
They are 1000 – 2000 nt long in prokaryotes
and 100-150 nt long in eukaryotes.
• The daughter strand consisting of
Okazaki fragments is called the
lagging strand.
63
Leading strand
Lagging strand
Fork movement
Leading strand
(continuous)
3'
5'
5'
3'
RNAase
P
OH
3'
5'
5'
3'
DNA polymerase
P
3'
5'
5'
3'
dNTP
DNAligase
3'
5'
5'
3'
ATP
• The replication of E. coli is
bidirectional from one origin, and the
two replication forks must meet at one
point called ter at 32.
• All the primers will be removed, and all
the fragments will be connected by
DNA-pol I and ligase.
 Nalidixic acid
 Novobiocin
 Ciprof loxacin
 Adriyamycin
 Etoposide
 Doxorubicin
INHIBITORS OF DNA REPLICATION
• DNAreplication is closely related with cell
cycle.
Eukaryotic Enzyme Prokaryotic Enzyme
DNA-pol : elongation DNA-pol III
DnaG,
primase
DNA-pol : initiate replication
and synthesize primers
DNA-pol : replication with
low fidelity
DNA-pol : Mitochondrial DNA synthesis
DNA-pol : lagging strand
synthesis, proofreading and
gap filling
DNA-pol I
Repair
⚫The eukaryotic replication origins are shorter than
that of E. coli. The ori-sites in Eukaryotes called
ARS (Autonomously Replicating Sequences) (or)
Replicators.
⚫Requires DNA-pol  (primase activity) and DNA-
pol  (polymerase activity and helicase activity).
⚫ DNA-pol  requires a protein called for its
activity Proliferating Cell NuclearAntigen (PCNA).
⚫Needs Topoisomerase and Replication factors (RF) to
assist.
• DNA replication and
nucleosome assembling occur
simultaneously.
• Overall replication speed is
compatible with that of
prokaryotes.
3'
5'
3'
5'
5'
3'
5'
3'
3'
5'
3'
5'
5'
3'
5'
3'
connection of discontinuous
segment
81
• The terminal structure of eukaryotic DNA
of chromosomes is called telomere.
• Telomere is composed of terminal DNA
sequence and protein.
• The sequence of typical telomeres is rich in
T and G.
• The telomere structure is crucial to keep
the termini of chromosomes in the cell
from becoming entangled and sticking to
each other.
82
• The eukaryotic cells use telomerase to maintain
the integrity of DNAtelomere.
• The telomerase is composed of
telomerase RNA
telomerase association protein
telomerase reverse transcriptase
• It is able to synthesize DNA using RNA as the
template.
83
Step in Replication Prokaryotic cells Eukaryotic cells
Recognition of origin of
replication
Dna A protein RpA
(Replication Protein-A)
Unwinding of DNA double helix Helicase
(requires ATP)
Helicase
(requires ATP)
Stabilization of unwound
template strands
Single-stranded DNA-binding
protein (SSB)
Single-stranded DNA-binding
protein (SSB)
Synthesis of RNA primers Primase Primase
Synthesis of DNA
Leading strand
Lagging strand
DNA polymerase III
DNA polymerase III
DNA polymerase δ
DNA polymerase Ԑ
Removal of RNA primers DNA polymerase I
(5 3' exonuclease)
RNAse-H
Replacement of RNA with DNA DNA polymerase I Unknown
Joining of Okazaki fragments DNA ligase
(requires NAD)
DNA ligase
(requires ATP)
Removal of positive supercoils
ahead of advancing
replication forks
DNA topoisomerase II
(DNA gyrase)
DNA topoisomerase II
2 dna replication pro & euk.

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2 dna replication pro & euk.

  • 1. HEENA KAUSAR Govt. E. Raghvendra Rao PG Science College
  • 2.  All organisms must duplicate their DNA with extraordinary accuracy before each cell division.  DNA replication is a biological process that occurs in all living organisms and copies their exact DNA. It is the basis for biological inheritance.  Replication is the process of synthesis of daughter DNA from parental DNA by the enzyme DNA Polymerase.  DNA templating is the process in which the nucleotide sequence of a DNA strand (or selected portions of a DNA strand) is copied by complementary base-pairing (A with T, and G with C) into a complementary DNA sequence.
  • 3. DNA RNA PROTEIN Transcription Translation Replication Reverse transcription
  • 5. ⚫A reaction in which daughter DNAs are synthesized using the parental DNAs as the template. ⚫Transferring the genetic information to the descendant generation with a high fidelity. Replication Parental DNA Daughter DNA 6
  • 6. 1. Semiconservative replication 2. Conservative replication 3. Dispersive replication
  • 9.  Semi-conservative replication  Bidirectional replication  Semi-continuous replication  High fidelity 10
  • 10.
  • 11. Cells broken open to extract DNA E. coli grown in the presence of 15N (a heavy isotope of Nitrogen) for many generations only 14N (a light isotope of Nitrogen) Sampled at: 0 min 1 • Cells get heavy-labeled DNA 2 E. coli placed in medium containing 3 40 min 20 min Suspended DNA in Cesium chloride (CsCl) solution. 4 15N medium
  • 12. CsCl density gradient centrifugation 5 15N 14N DNA Both strands heavy F1 generation DNA (one heavy/one light strand) 0 min 20 min 40 min F2 generation DNA:  Two light strands  One heavy/One light strand
  • 13.
  • 16. Half of the parental DNA molecule is conserved in each new double helix, paired with a newly synthesized complementary strand. This is called semiconservative replication.
  • 17.
  • 18. • Replication starts from unwinding the dsDNA at a particular point (called origin / ori site), followed by the synthesis on each strand. • The parental dsDNA and two newly formed dsDNA form a Y-shape structure called Replication fork.
  • 19.
  • 20. The replication process starts from the origin, and proceeds in two opposite directions. It is named - Replication. 21
  • 21. • DNA Polymerase - Matches the correct nucleotides then joins / polymerizes adjacent nucleotides to each other. • Helicase - Unwinds the DNA and melts it. • Primase - Provides an RNA primer to start polymerization.
  • 22. • Single Strand Binding Proteins - Keep the DNA single stranded after it has been melted by helicase • Gyrase - A topisomerase that Relieves torsional strain in the DNAmolecule. • Ligase - Joins adjacent DNA strands together (fixes “nicks”) • Telomerase - Finishes off the ends of DNA strands in Eukaryotes
  • 23. DNA Polymerase-I • The first DNA- dependent DNA polymerase ( DNA Pol -I ) was discovered in 1958 by Arthur Kornberg who received Nobel Prize in physiology & medicine in 1959. • DNA Polymerase is considered as Kornberg Enzyme.
  • 24. • Later, DNA-Pol II and DNA-Pol III were identified. • All of them possess the following biological activity. • 53 Polymerse activity • Exonuclease activity
  • 25. 3´→5´ exonuclease activity excise mismatched nuleotides A G G A A A G T C C G G C G 5´→3´ exonuclease activity removes primer or excise mutated segment 5' C T T C 3' 3' G 5'
  • 26. ⚫Mainly responsible for proofreading and filling the gaps, repairing DNA damage 30
  • 27. • Small fragment (323 AA): having 5´→3´ exonuclease activity • Large fragment (604 AA): called Klenow fragment, having DNA polymerization and 3´→5´exonuclease activity Large fragment Small fragment C-end DNA-pol Ⅰ Cleavage
  • 28. • Temporarily functional when DNA-pol I and DNA-pol III are not functional. • Still capable for doing synthesis on the damaged template. • Participates in DNArepair process.
  • 29. • A heterodimer enzyme composed of ten different subunits • Having the highest polymerization activity (105 nt/min) • The true enzyme responsible for the elongation process
  • 30. α: has 5´→ 3´ polymerizing activity ε:has 3´→ 5´ exonuclease activity and plays a key role to ensure the replication fidelity. θ: maintain heterodimer structure
  • 31.
  • 32.
  • 34.
  • 35. • Also called DnaG • Primase is able to synthesize primers using free NTPs as the substrate and the ssDNAas the template. • Primers are short RNA fragments of a several nucleotides long.
  • 36.
  • 37. • Primers provide free 3´-OH groups to react with the -P atom of dNTP to form phosphodiester bonds. • Primase, DnaB, DnaC and an origin form a Primosome complex at the initiation phase.
  • 38. • Also referred to as DnaB. • It opens the double strand DNAwith consumingATP. • The opening process with the assistance of DnaAand DnaC
  • 39. • Single Strand DNABinding protein. • SSB protein maintains the DNA template in the single strand form in order to • prevent the dsDNAformation; • protect the vulnerable ssDNA from nucleases.
  • 40. • It cuts phosphoester bonds on both strands of dsDNA, releases the supercoil constraint, and reforms the phosphodiester bonds. • It can change dsDNA into the negative supercoil state with consumption of ATP.
  • 42. • Connect two adjacent ssDNA strands by joining the 3´-OH of one DNA strand to the 5´-P of another DNA strand. • Sealing the nick in the process of Replication, Repairing, Recombination, and Splicing.
  • 43. • Replication based on the principle of base pairing is crucial to the high accuracy of the genetic information transfer. • Enzymes use two mechanisms to ensure the replication fidelity. –Proofreading and real-time correction –Base selection
  • 44. • DNA-pol I has the function to correct the mismatched nucleotides. • It identifies the mismatched nucleotide, removes it using the 3´- 5´ exonuclease activity, add a correct base, and continues the replication.
  • 45.
  • 47. 1) Initiation • Occurs at the origin of replication • Separates dsDNA, primer synthesis 2) Elongation • Involves the addition of new nucleotides (dNTPs ) based on complementarity of the template strand • Forms phosphoester bonds, correct the mismatch bases, extending the DNAstrand, … 3) Termination • Stops the DNAReplication occurs at a specific termination site
  • 48. • The replication starts at a particular point called origin of Replication (or) ori-Site. • The structure of the origin is 248 bp long andAT-rich. 9 mer- sequence 13 mer- sequence
  • 49.
  • 50. Site where DNA synthesis starts
  • 51. • DnaArecognizes ori C. • DnaB ( Helicase ) and DnaC join the DNA- DnaA complex, open the local AT-rich region, and move on the template downstream further to separate enough space. • DnaAis replaced gradually. • SSB protein binds the complex to stabilize ssDNA.
  • 52. • Primase joins and forms a complex called primosome. • Primase starts the synthesis of primers on the ssDNA template using NTP as the substrates in the 5´- 3´ direction at the expense ofATP. • The short RNA fragments provide free 3´-OH groups for DNA elongation.
  • 53. Primase synthesizes PRIMER ’ Single stranded binding protein Initiation
  • 54. ⚫dNTPs are continuously connected to the primer or the nascent DNA chain by DNA-pol III. ⚫The core enzymes (、、and  ) catalyze the synthesis of leading and lagging strands, respectively. ⚫The nature of the chain elongation is the series formation of the phosphodiester bonds.
  • 55.
  • 56. 3’ 3’ Laging strand 5’ Okazaki fragments Gap filled byDNA Ligase Pri E m lo en rg is at rie om no bv y eD dNb A yP D oN lyA mP er oa ly se m Ie II rase I
  • 57. • RNA Primers on Okazaki fragments are digested by the enzyme RNase. • The gaps are filled by DNA-pol I in the 5´→3´direction. • The nick between the 5´end of one fragment and the 3´end of the next fragment is sealed by ligase.
  • 58. • Many DNA fragments are synthesized sequentially on the DNA template strand having the 5´- end. These DNA fragments are called Okazaki fragments. They are 1000 – 2000 nt long in prokaryotes and 100-150 nt long in eukaryotes. • The daughter strand consisting of Okazaki fragments is called the lagging strand. 63
  • 61.
  • 63. • The replication of E. coli is bidirectional from one origin, and the two replication forks must meet at one point called ter at 32. • All the primers will be removed, and all the fragments will be connected by DNA-pol I and ligase.
  • 64.  Nalidixic acid  Novobiocin  Ciprof loxacin  Adriyamycin  Etoposide  Doxorubicin INHIBITORS OF DNA REPLICATION
  • 65.
  • 66. • DNAreplication is closely related with cell cycle.
  • 67.
  • 68. Eukaryotic Enzyme Prokaryotic Enzyme DNA-pol : elongation DNA-pol III DnaG, primase DNA-pol : initiate replication and synthesize primers DNA-pol : replication with low fidelity DNA-pol : Mitochondrial DNA synthesis DNA-pol : lagging strand synthesis, proofreading and gap filling DNA-pol I Repair
  • 69. ⚫The eukaryotic replication origins are shorter than that of E. coli. The ori-sites in Eukaryotes called ARS (Autonomously Replicating Sequences) (or) Replicators. ⚫Requires DNA-pol  (primase activity) and DNA- pol  (polymerase activity and helicase activity). ⚫ DNA-pol  requires a protein called for its activity Proliferating Cell NuclearAntigen (PCNA). ⚫Needs Topoisomerase and Replication factors (RF) to assist.
  • 70. • DNA replication and nucleosome assembling occur simultaneously. • Overall replication speed is compatible with that of prokaryotes.
  • 72. • The terminal structure of eukaryotic DNA of chromosomes is called telomere. • Telomere is composed of terminal DNA sequence and protein. • The sequence of typical telomeres is rich in T and G. • The telomere structure is crucial to keep the termini of chromosomes in the cell from becoming entangled and sticking to each other. 82
  • 73. • The eukaryotic cells use telomerase to maintain the integrity of DNAtelomere. • The telomerase is composed of telomerase RNA telomerase association protein telomerase reverse transcriptase • It is able to synthesize DNA using RNA as the template. 83
  • 74.
  • 75. Step in Replication Prokaryotic cells Eukaryotic cells Recognition of origin of replication Dna A protein RpA (Replication Protein-A) Unwinding of DNA double helix Helicase (requires ATP) Helicase (requires ATP) Stabilization of unwound template strands Single-stranded DNA-binding protein (SSB) Single-stranded DNA-binding protein (SSB) Synthesis of RNA primers Primase Primase Synthesis of DNA Leading strand Lagging strand DNA polymerase III DNA polymerase III DNA polymerase δ DNA polymerase Ԑ Removal of RNA primers DNA polymerase I (5 3' exonuclease) RNAse-H Replacement of RNA with DNA DNA polymerase I Unknown Joining of Okazaki fragments DNA ligase (requires NAD) DNA ligase (requires ATP) Removal of positive supercoils ahead of advancing replication forks DNA topoisomerase II (DNA gyrase) DNA topoisomerase II