Lecture 4 - DNA Repair

Question 1

What is the Ames test used for? Explain how it works.

Answer 1

To test the mutagenic potential of a chemical aka whether its a potential carcinogen

1. Start with a strain of bacteria that has a mutation in the gene required for His synthesis (aka requires external His to survive) and plate them with minimal His media
2. Add mutagen to one and the other is the control
3. Few colonies grow on the control: natural revertants (spontaneously mutate to produce His) but many grow on the other because were able to mutate to synthesis His

Question 2

What is another way of saying carcinogen?

Answer 2

Cancer-causing agent

Question 3

What happens when too much mutagen is added to the plate in the Ames test?

Answer 3

Too high concentration can be lethal

Question 4

What is the purpose of DNA repair?

Answer 4

To repair post-replication mutations

Question 5

How often do accidental base changes in DNA result in a permanent mutation?

Answer 5

Less than 1 in 1000

Question 6

Why does DNA methylation occur?

Answer 6

Many reasons but mainly gene expression regulation = epigenetics

Question 7

Where does methylation and mismatch repair primarily happen?

Answer 7

Prokaryotes

Question 8

Where is DNA methylated in both prokaryotes and eukaryotes?

Answer 8

At the N6 of adenines in (5′)GATC sequences, which are palindromes present in opposite orientations on the two strands

Question 9

How does methylation help mismatch repair post-replication? How is the DNA referred to at this time?

Answer 9

Following replication, the new daughter strand for a short period of time, is not methylated = hemimethylated DNA

The repair mechanisms need to know which is the parent and which is the daughter because if there is a mismatch they want to repair the daughter strand as the parent one is a high fidelity template

Question 10

What enzyme methylates the daughter strand post-replication? Can the daughter and parent strand be distinguished at this point?

Answer 10

Dam methylase

NOPE

Question 11

Describe post-replication mismatch repair. 6 steps

Answer 11

1. Proteins MutS and MutL recognize a mismatch and form a complex on the DNA using ATP
2. DNA is threaded through the complex until it reaches MutH bound at a DNA methyl group to identify the parent strand (usually about 12 base pairs before reaching one)
3. MutH cleaves the unmethylated strand on the 5′ side of the G in this sequence
4. A complex consisting of DNA helicase II and one of several exonucleases then degrades the unmethylated DNA strand from that point to just beyond the mismatch
5. DNA Pol III adds the correct bases
6. Nick is sealed by DNA ligase

Question 12

What determines what kinds of exonucleases are used during post-replication mismatch repair?

Answer 12

Whether the daughter strand was cleaved on the 3’ or 5’ side of the mismatch

Question 13

Why is our DNA a target for spontaneous modifications? How frequent are these?

Answer 13

Because it resides in an aqueous environment where other chemicals reside and can make spontaneous modifications to it

VERY frequent

Question 14

What are 4 example of spontaneous modifications of DNA?

Answer 14

1. Oxidative damage
2. Hydrolytic attacks: depurination and deamination
3. Uncontrolled methylation by S-adenosylmethionine
4. UV damage causing dimerization of adjacent Ts

Question 15

What is depurination of DNA?

Answer 15

An entire base is removed from a nucleotide

Question 16

How often does DNA depurination happen?

Answer 16

5000 x / cell / day

Question 17

What happens during deamination?

Answer 17

NH3 is removed and replaced with C=O

Question 18

What happens if you deaminate a C base?

Answer 18

You get a U

Question 19

What happens if you deaminate a 5’-methylated C base?

Answer 19

You get a T

Question 20

What happens if you deaminate an A base?

Answer 20

You get hypoxanthine

Question 21

What happens if you deaminate a G base?

Answer 21

You get xanthine

Question 22

Which deamination is an epigenetic mutation?

Answer 22

Deamination of 5-methylcytosine to thymine

Question 23

Which deamination is the most common? How is it repaired?

Answer 23

Deamination of cytosine to uracil

Base excision repair

Question 24

What are the 2 ways in which UV light dimerizes T residues?

Answer 24

1. Results in formation of a cyclobutyl ring involving C-5 and C-6 of adjacent T residues = cyclobutane pyrimidine dimer => introduces a kink in DNA
2. Results in a 6-4 photoproduct, with a linkage between C-6 of one T and C-4 of its neighbor T

Question 25

What is most easily recognized by DNA repair mechanisms?

Answer 25

Deformations of the DNA helix

Question 26

What can also cause T dimerization other than UV?

Answer 26

Cigarette smoking

Question 27

How are T dimers repaired? Describe the mechanism.

Answer 27

Nucleotide excision repair

1. Excision nuclease nicks the strand with the dimer several nucleotides away on both sides of the dimerization
2. Helicase removes that chunk of the strands
3. DNA polymerase I/epsilon replaces the nucleotide gap (and some) using the 3’ free (-OH) on the nick of the strand as a primer
4. DNA ligase seals nick

Question 28

How are spontaneous DNA alterations repaired?

Answer 28

Excision repair

Question 29

What are the 2 types of excision repairs?

Answer 29

1. Base excision repair

2. Nucleotide excision repair

Question 30

How can spontaneous DNA alterations result in a sustained mutation?

Answer 30

If deamination or depurination has occured, DNA replication will create one unchanged daughter strand and one mutated strand with the correct base pair added (for deamination) or a point deletion (for depurination)

Question 31

Are the consequences of a sustained mutation more severe in a germ cell or in a somatic cell. Why?

Answer 31

Germ cell because it’ll be reproduced indefinitely

Question 32

Describe the mechanism of base excision repair.

Answer 32

1. DNA glycosylase recognizes an incorrectly pairs base and cleaves it off
2. AP endonuclease + phosphodiesterase removes the leftover phosphodiester backbone along with its ribose
3. DNA polymerase I starts synthesis from the free 3′ hydroxyl at the nick, removing (with its 5′→3′ exonuclease activity) and replacing a portion of the damaged strand using the 3’ free (-OH) on the nick of the strand as a primer
4. DNA ligase seals nick

Question 33

What does the length of the DNA chunk removed during nucleotide excision repair dependent on?

Answer 33

Whether it’s in eukaryotes (longer) or prokaryotes (shorter)

Question 34

Is the repair of double strand breaks typically complete?

Answer 34

NOPE

Question 35

Are double strand breaks less or more common than spontaneous DNA alterations?

Answer 35

Less

Question 36

What are the 2 mechanisms to repair DNA double strand breaks? When is each used? Which one predominates?

Answer 36

1. Nonhomologous end joining: somatic cells - PREDOMINATES
2. Homologous recombination: can only be used shortly after replication when there is a sister chromatid available to serve as the template (in S and G2 phases of the cell cycle)

Question 37

Describe the mechanism of nonhomologous end joining and the resulting DNA. 3 steps

Answer 37

1. End is recognized by Ku heterodimers and other proteins (eg: p53 and BRCA1) that bind to prevent degradation of the DNA and arrest the cell cycle
2. Nucleotides are chewed back to remove the nucleotide overhand that results from the break until a blunt end is obtained
3. Ends are joined by DNA ligase

Resulting DNA has suffered nucleotide deletions

Question 38

Why is it important for the cell cycle to be arrested during nonhomologous end joining?

Answer 38

So that the cells do not divide and propagate the mutation

Question 39

What can cell cycle dysfunction and propagation of mutated cells that lead to cancer be due to?

Answer 39

p53 and BRCA1 gene mutations

Question 40

Describe the mechanism of homologous recombination and the resulting DNA. 5 steps

Answer 40

1. Exonucleases degrade the 5’ ends of each DNA strand leaving 3’ overhangs
2. Strand invasion: a single broken strand will crossover to the sister chromatid at a branch point
3. Branch point migrates along the length of the sister chromatid so that the template can be read and DNA polymerase can synthesize a new strand portion
4. The newly synthesized DNA pairs with the top-strand and DNA synthesis finishes
5. DNA ligase joins the ends

Resulting DNA: break COMPLETELY repaired

Question 41

What does a mutation in BRCA2 affect? What does it cause?

Answer 41

Affects repair by homologous recombination

Causes breast, ovarian, and prostate cancer

Question 42

What does a mutation in MSH2, 3, 6, MLH2, PMS2 affect? What does it cause?

Answer 42

Affects mismatch repair

Causes colon cancer

Question 43

What does a mutation in xeroderma pigmentosum (XP) groups A-G affect? What does it cause?

Answer 43

Affects nucleotide excision repair

Causes skin cancer, UV sensitivity, neurological abnormalities

Question 44

What do a lot of inherited syndromes with defects in DNA repair cause?

Answer 44

Cancer

Question 45

What does a mutation in XP variant affect? What does it cause?

Answer 45

Translesion synthesis by DNA polymerase

Causes skin cancer, UV sensitivity

Question 46

What does a mutation in ataxia telanglectasia (AT) affect? What does it cause?

Answer 46

ATM protein, kinase activated by double-stranded breaks

Causes leukemia, lymphoma, gamma-ray sensitivity, genome instability

Question 47

What does Werner syndrome affect? What does it cause?

Answer 47

Accessory 3’-exonuclease and DNA helicase

Causes premature aging, cancer at several sites, genome instability

Question 48

What does Bloom syndrome affect? What does it cause?

Answer 48

Accessory DNA helicase for replication

Causes cancer at several sites, stunted growth, and genome instability

Question 49

What do Fanconi anemias groups A-G affect? What does it cause?

Answer 49

DNA interstrand cross-link repair

Causes congenital abnormalities, leukemia, and genome instability

Question 50

What does a 46 BR patient have affected? What does this cause?

Answer 50

DNA ligase I

Causes hypersensitivity to DNA-damaging agents, genome instability

Question 51

What happens when BRCA 1 is completely deficient?

Answer 51

1. Impaired DNA damage repair
2. Defective G2/M cell cycle checkpoint
3. Centrosome amplification

==> Genetic instability leading to either:

• p53 activation => cell cycle arrest OR apoptosis => development abnormalities or embryonic lethality
• p53 inactivation => activation of oncogenes => clonal expansion => tumorigenesis

Question 52

What is the Peto paradox?

Answer 52

You would think that as animals get bigger and have more cells and as their lifespan gets longer they would have a higher cancer incidence, but this is not true.

The incidence of cancer is remarkably flat

Question 53

What is the human cancer mortality?

Answer 53

11-25%

Question 54

What is the elephant cancer mortality?

Answer 54

4.8%

Question 55

What can explain the Peto paradox?

Answer 55

Larger animals with more cells have more genes that code for binding proteins that bind DNA for repair like p53 without which apoptosis does not occur and cancer does instead

Question 56

What is a retrogene?

Answer 56

DNA copy of the RNA that is reinserted as a gene (aka a gene without introns)

Question 57

How many alleles for TP53 in humans vs elephants? What does this mean for human vs elephant cells?

Answer 57

Humans: 2
Elephants: 40 (including 38 retrogenes)

Elephant cells more readily undergo apoptosis

Question 58

Difference between exonucleases and endonucleases?

Answer 58

Exonuclease causes the hydrolysis of a nucleotide at the ends where a free 3’ or 5’ hydroxyl group is present in the polynucleotide chain while the exonuclease does not require a free 3’ or 5’ hydroxyl group to cause hydrolysis of the polynucleotide chain.