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Transcript 
Lecture 25: DNA mutation,
proofreading, and repair
G
C
A
T
T
A
1 nm
C
G
C
3.4 nm
G
A
T
G
C
T
A
T
A
A
T
T
A
G
A
Figure 16.7a, c
C
0.34 nm
T
(c) Space-filling model
1
Lecture Outline 11/2/05
•
•
•
•
Review DNA replication machine
Fidelity of replication and proofreading
Replicating the ends of chromosomes
Mutation
– Types of mutations
– Repair mechanisms
2
DNA synthesis goes 5’ to 3’
• DNA
New strand Template strand
polymerases,
3 end
5 end
add nucleotides
to the 3 OH at
Sugar
A
T
Base
the end of a
Phosphate
growing strand
C
G
G
C
OH
A
C
OH
5 end
Figure 16.13
Nucleoside
triphosphate
P
P
Pyrophosphate
3
Model for the “replication machine,” or replisome
4
Peter J. Russell, iGenetics: Copyright © Pearson Education, Inc., publishing as Benjamin Cummings.
Replication overview
• Look at animations on your textbook CD
• Look again at the animation from DNAi
– http://www.dnai.org
– (go to the section on copying the code)
5
DNA Polymerase III
• A complex enzyme with many subunits
•
one part adds the nucleotides
•
another helps it slide along the template
•
another checks for mis-pairing
6
Figs. from http://www.mun.ca/biochem/courses/3107
Proofreading
• Even though bases preferentially pair G-C and A-T,
the initial error rate is about 1 in 10,000.
• Many polymerases have “proofreading” ability. They
can excise an mis-paired base and try again.
• This reduces the error rate to about 1 in a million.
One polymerase subunit adds nucleotides
Another “edits” out incorrect7 bases
Fidelity of replication
Replication step
error rate
5′→3′ polymerization
1 × 105
3′→5′ proofreading
1 × 102
Strand-directed mismatch repair 1 × 102
Total error rate
1 × 109
8
What happens to the lagging strand
at the very end of the chromosome?
Leaves a gap when the RNA
primer is removed
3’
5’
5’
3’
3’
5’
9
The ends of eukaryotic chromosomal DNA get
shorter with each round of replication
5
Leading strand
Lagging strand
End of parental
DNA strands
3
Last fragment
Previous fragment
RNA primer
Lagging strand
5
3
Primer removed but
cannot be replaced
with DNA because
no 3 end available
for DNA polymerase
Removal of primers and
replacement with DNA
where a 3 end is available
5
3
If they get short enough,
essential genes will
eventually be deleted
Second round
of replication
5
New leading strand 3
New lagging strand 5
3
Further rounds
of replication
Figure 16.18
Shorter and shorter
daughter molecules
10
Telomerase
Carries its own RNA
template
Extends the old
(template) strand
Normal synthesis of
new DNA
11
What happens to the lagging strand
that the end of the chromosome?
• Telomeres contain hundreds of simple tandem repeats.
• In humans, the repeat sequence is TTAGGG
TTAGGG TTAGGG TTAGGG TTAGGG TTAGGG . . . . . . .
Lots of junk, so if the ends get slightly shorter, no essential genes are lost
• Cell lines with active telomerase live longer than those without
telomerase.
– That may be important in allowing cancer cells to continue to divide.
12
Mutations and repair
13
Various kinds of mutations:
Purine -> Purine or Pymimidine -> Pyrimidine: common
Purine -> Pymimidine: rare
Some mutations change the code to a new amino acid
14
Types of base pair substitutions and mutations.
Others are silent
Additions and deletions
15
Mutations can be caused by:
•
•
•
•
Chemical mutagens
Ionizing radiation
Slippage during DNA replication
Spontaneous errors
16
Chemical changes in one of the
nucleotide bases
After replication, new strand has an A
Deamination changes C to U
--C----G---
--U----G---
--U----A---
--T----A---
--G----C---
17
UV damage (e.g. pyrimidine dimers)
UV radiation can
cause thymine
dimers
18
19
• In nucleotide excision repair
– Enzymes cut out and replace damaged
stretches of DNA
1 A thymine dimer
distorts the DNA molecule.
2 A nuclease enzyme cuts
the damaged DNA strand
at two points and the
damaged section is
removed.
Nuclease
DNA
polymerase
3 Repair synthesis by
a DNA polymerase
fills in the missing
nucleotides.
DNA
ligase
Figure 16.17
4 DNA ligase seals the
Free end of the new DNA
To the old DNA, making the
strand complete.
20
Certain bacterial mutations
cause increased mutation rates
Defect in:
Rifr mutants per 108 cells
Wild-type (mut+ )
5-10
Pol III proofreading
(mutD)
Mis-match repair
(mutS)
Base excision repair
(mutY mutM)
4000-5000
760
8200
21
Mismatch repair
Here is a mis-paired base that must be
repaired:
G
T
How is the mistake recognized?
How does the mismatch repair system
know which strand is the new one and
which strand is the old one?
22
MutS/L/H
Certain enzymes detect the
deformed helix that results from the
incorrect pairing
G
T
The old (template) DNA
has methyl groups in
certain places
MutS/L/H
G
T
CH3
GATC
CTAG
Cut the newly
synthesized strand
here
23
G
CH3
GATC
G
DNA pol I/III
DNA Ligase
Re-synthesize DNA from the
template using the normal DNA
polymerases
CH3
G
C
GATC
CTAG
Corrected base pair
24
• Various similar
mechanisms for
other types of
mutations
25
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