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DNA Synthesis

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Title: DNA Synthesis

1
DNA Synthesis
Lecture 31
Mukund Modak, Ph.D.
2

DNA Objectives
Define a DNA polymerase reaction and its
components.
Where does DNA replication begin? Where does it
terminate?
Know about leading and lagging strand synthesis.
How many primers are required for each strand
synthesis?
What are Okazaki fragments? Remember some of the
components required in lagging strand synthesis
such as Pol I to remove RNA primers and DNA
ligase to join the Okazaki fragments.
Know the polarity of DNA to be replicated.
Know the major eukaryotic DNA polymerases.
Remember clamp protein( PCNA in eukaryotes and B
clamp in prokaryotes) that clamps DNA pol (
mainly delta and epsilon) to template and speeds
up polymerase rate.
What does enzyme telomerase do? It has RNA
component with sequence complimentary to
telomeric( DNA) sequences.

3
Watson-Crick Model
Base

Double helix
Antiparallel
Base-paired
Base stacking
Major groove
Minor groove
Sugar-phosphate
Backbone
Helix structure by X-ray diffraction

3
2
O
P
Base
O
5
O
P
Base
Postulations Semi conser- vative replication via
base pairing principle. Expression via
transcription (by same base pairing rule)
O
5
3
4
Review of Basics

DNA replication is semiconservative

5
Review of Basics

DNA is synthesized by the addition of a
deoxynucleotide to the 3? end of a polynucleotide
chain
Base-pairing between incoming dNTP and template
strand provides specificity

6
Antiparallel Double Strand
5
3
5
3
Base
Polymerization reaction
O
5
OH 5 PPP 3O - P - 5O PPi
3
P-P-P-O-H2C
Therefore chain extends 3 to 5 Overall
growth 5 to 3
3
OH
Base
O
5
5
3
P-P-P-O-H2C
OH
5P
New chain
3
5P
OH
5
3
OH
7
DNA dependent DNA polymerases are key enzymes for
DNA synthesis Requirements Template, primer,
4dNTPs, Mg 2
? Nucleotidyl transferase reaction ? Template
dependent dNTP selection ? direction of
synthesis 5 ? 3
Imp Primer (DNA or RNA) with 3OH, a minimum of
10 bases hydrogen bonded to template
5
3
3OH
3OH
3OH
5
5
5
Enzyme
Mg.dNTP
Primer n1 PPi
Prokaryotes contain 3 DNA polymerases I, II and
III
8
Specialized enzymes and factors

Specialized polymerases that synthesize primers
and DNA
Editing exonucleases to work with polymerases.
Topoisomerases that convert supercoiled DNA to
relaxed form
Helicases that separate two parental strands of
DNA
Accessory proteins promoting tight binding of
polymerase to DNA and
thereby increase the speed of polymerases
(sliding clamps)
Details of the process

9
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10
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11
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12
Leading vs Lagging Strand Replication
3
13
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14
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15
DNA REPLICATION PROTEINS
dnaA Ori C dnaB begins unwinding
(helicase) Rep Helicase Ongoing
unwinding SSB Stabilize ss DNA Gyrase
and Topoisomerase Supercoil to relax
transition Primase Synthesis of primer
(RNA) Pol III complex DNA synthesis Pol
I Primer removal and gap filling DNA
ligase Join DNA ends Topo IV Decatenates
replicated circles
Topo IV
16
REPLICATION FORK SUMMARY
Begins with unwinding of two strands with
opposite polarity Two replisome assemblies
(Primase Pol III complex) Leading strand
(continuous synthesis) Lagging strand
(discontinuous synthesis) a. Looping of the
strand to transiently change polarity and
permit primer synthesis b. DNA synthesis in
pieces (Okazaki fragments) c. Pol I to remove
RNA primers and replace by DNA d. DNA ligase to
join small DNAs into a single large molecule
with ATP or NAD as a cofactor Termination
signal TUS factor Two forks reach each other at
mid point of the circle and are stalled by TUS
factor Replication completes with generation of
catenated circles. Seperation of circles by Topo
IV
17
PROOF READING ACTIVITY OF POL I (3 to 5
exonuclease activity)
18
Structure of first DNA polymerase (Klenow
Fragment of E.coli pol I, 1985)
Nomenclature of various structural units
(1992) Thumb Palm Fingers 3 5 exonuclease
The crystal structures of numerous DNA
polymerases solved later, showed same general
anatomy
19
Lecture 8
20
Eukaryotic DNA replication
G0, G1, S and M Phases (DNA replication in S
phase)
Many polymerases and accessory factors required
Multiple initiation points to replicate (3
billion bps) Linear chromosome Overall
replication scheme similar to prokaryotes Problem
with 5 RNA primer removal and fill
up Solution to this problem is telomerase action
21
Eukaryotic DNA Polymerases

a Repair and Replication and primase function
Repair function
g Mitochondrial DNA polymerase
d Replication with PCNA (processivity factor)
Replication
? Repair function
i Repair function

Telomerases
Terminal deoxynucleotidyl transferase Viral
reverse transcriptase Viral replication
22
Eukaryotic Fork

Three polymerases required for replication
Pol? synthesizes primer RNA and very little DNA
(non-processive, no proofreading exonuclease)
Pol? and Pol? both are processive (interact with
PCNA) and have proofreading exonucleases

23
Important Participants In Eukaryotic DNA
Replication

Pol (alpha) (delta) and (epsilon) primer
synthesis and DNA synthesis (There is a separate
primase in prokaryores)
Sliding clamp or processivity factor PCNA
Increases rates and length of DNA (Equivalent to
ß clamp in prokaryotes)
FEN-1 nuclease removes RNA primers (In
prokaryotes, 5- nuclease activity of pol I does
it)
RPA is a single strand binding protein (SSB in
prokaryotes)