Sources and consequences of genomic instability

Question 1

For each type of break, what is there?

Answer 1

Specific tool kit and within that tool kit there are some shared components.

Question 2

Is DNA stable?

Answer 2

Very stable inside the cell.
Very unstable outside the cell.

Question 3

Why is DNA unstable within the cell?

Answer 3

Reactive oxidative species and enzymes mean DNA becomes unstable.

~7 lesions cell minute.

Question 4

When are DNA breaks good?

Answer 4

When in an programmed way.

Immunoglobulin diversity. Fight infections. Introducing breaks and reshuffling the viable region in antibody to produce/develop antibody for each infection.

Meiosis: generate diversity in population by introducing break, reshuffling DNA between parents.

Turn on and off gene expression.

Introduce a break, conformation of that circuit changes and closes on itself. Change can be expressed.

Question 5

What are the consequences of un-repaired DNA damage?

Answer 5

Cell death (degenerative disease and autoinflammation and cell survival (cancer)

Breaks exceed certain threshold.

If you have lots of cell death due to unrepaired breaks.

Causing degeneration in organs. Most affected organ is the nervous system.

Autoinflammation.

Question 6

What is another consequence of un-repaired DNA break?

Answer 6

Other consequence is that cells may decide to continue dividing (cell survival) in presence of DNA break. Induce mutations and then cause cancer.

Question 7

Link between genetic instability and cancer

Answer 7

See enrichment of mutations in protein-coding genes involved in DNA damage response (DDR).

Mess up DNA repair = cancer.

Question 8

How might disease of the nervous system arise?

Answer 8

Only born with certain number neurons, exposed to various stresses. Those neurons if they accumulate damage in DNA by time function will be compromised. Causing disease in nervous system.

People living linger is increasing, putting pressure on health system.

Question 9

What threatens genomic integrity?

Answer 9

Impaction – generate lots of supercoiling, tangling which needs to be unwinded.

If they were to transcribe to RNA, replicate during cell devision and there is recombination.

Done by enzymes topisomerese – these enzymes unwind. Do this dangerously by introducing a break in one or two strands of double helix. Then allow swivelling of other strand around the transient nick.

Question 10

Oxidative and protein-linked DNA breaks

Answer 10

Reactive oxygen species

DNA topoisomerase

By-products during demethylation of histones and DNA (formaldehyde).

Question 11

What is the concept behind impaction threatening genomic integrity.

Answer 11

Concept – there are enzymes in the cell that are very important to relax super coiling, during process they can break. End up with bit of protein stuck on DNA termini.

Question 12

How does gene transcription - Epigenetic re-programming at regulatory regions producs ROS (very new) - pose a threat to genomic integrity?

Answer 12

Histone demethylation and DNA demethylation.

During cell transcription activation you need to remove certain silencing marks, histones are methylated. Need to remove methyl group on histones to turn on genes.

As a by product of demethylation you can produce oxidative stress.

Same happens ensuring DNA methylation.

Methyl cytosine? Common epigenetic mark which prevents gene expression. To turn of gene expression you need to remove the methyl group from 5-methyl cytosine. This is done by methylases and as a by product is generates ROS.

Question 13

What is the main concept behind turning on gene expression?

Answer 13

Understand concept of that during turning on gene expression you need to remove methyl groups from histone from DNA. During demethylation ROS are produce as a by product and go on and damage nearby DNA.

Question 14

Does DNA replication pose a threat to genomic integrity? How? (add this)

Answer 14

Yes

Question 15

Epigenetic re-programming in the non-coding genome produces ROS.

Answer 15

Those types of reprogramming during gene activation are most pronounced gene regulatory elements.

The bit that is very vulnerable to this type of damage is the regulatory region, not necessarily the protein coding region. The non-coding region, ie promotor and enhancers – these regions have the most methylation events.

Question 16

How is gene transcription a threat to DNA integrity?

Answer 16

Due to demethylation events.

RNA polymerase travelling across gene to transcribe to make RNA – this RNA can pair back to DNA.

DNA is double helix and RNA generated by RNA polymerase is one strand - end up with three strand happening all time during gene transcription.

Issue because a strand becomes exposed therefore vulnerable to breakage and easily broken – R-loops.

Question 17

Why is the speed of polymerase important in gene transcription?

Answer 17

Id transcription is fast there will be no chance for R-loops to form. But anything that slows down the travelling polymerase will increase chance of this tearing RNA with the DNA and formation of R-loops.

Slow down polymerase = increased propensity of R-loop formation.

Transcription by products = R-loops

Question 18

What are physiological and pathological consequences of R-loops?

Answer 18

Long regions of exposure.

Longer genes are more prone to this – they polymerase sits longer on them.

Question 19

Why might a polymerase slow down?
State a pathological disorder

Answer 19

If polymerase encounters lots of repetitive regions, gets confused. Polymerase slows down.

Where can you find repetitive sequences on DNA?

Centromeres, telomeres, CpG islands, Start of genes which are CpG rich, ribosomal DNA (most repetitive in sequence DNA).

Pathological – Polynucleotide repeat expansion disorders – several ataxias, Huntingtons, MND.

Question 20

How does ribose contamination cause DNA instability?

Answer 20

DNA in full of ribose (suppose to be in RNA).

Different between deoxyribose and ribose in a oxygen.

Reason DNA is full of ribose is that the oxygen, electrons attack phosphodiester bond, bond always broken due to the oxygen – makes RNA very unstable.

So why do we have lots of ribose in DNA? Because the building block the pool of ribonucleotides

Specific repair pathways which deal with this.

Question 21

What are the physiological and pathological consequences of r-loops?

Answer 21

They can be useful to guide the termination of transcripts.
They can relieve topological constraines and supercoiling
A major source of DNA breaks if left un-resolved.

Question 22

Spontaneous base loss.

Answer 22

Labile under physiological conditions (hydrolysis)

~ 18000 purines

~ 600 pyrimidines

Per diploid genome per day

Cause abasic sites – a problem which induces mutations.

Question 23

Endogenous base modifications - deaminations

Answer 23

In cytosine, if you lose a amino group it becomes a uracil. During second round of replication, the upper strand will pair A instead of G. – Transition mutation which is caused by loss of amino group.

Deamination of meC is major cause of mutation in human cancers e.g p53 mutations

Under representation of CG in the genome.

Question 24

Base modification - Base oxidation

Answer 24

By products of normal aerobic metabolism = reactive oxygen species (ROS)

Singlet oxygen, peroxide radicals, hydrogen peroxide and hydroxyl radicals

Over 80 different products known – reacts with double bonds – ROS also produce single strand breaks and lipid peroxidation.

Example – guanine converted to 8-oxoG which can pair with C or A.

Problem because it mis-pairs. Cause a C to A transition mutation.

Question 25

Concept behind base modification impact DNA integrity?

Answer 25

Concept – if you deaminate a base you have a mispairing

If you oxidise a base you have a mispairing

Question 26

Other than to the bases, what else is affected by oxidation?

Answer 26

Ribose

When ribose is oxidised it fragments.

That causes lots of weird chemistry in ribose.

For example – alpha-keto-aldehyde (don’t necessarily need to learn),

All are product of sugar being hit via ROS that fragments and the remaining of the sugar is then attached to DNA termini.

Question 27

Methylation and alkylation

Answer 27

Endogenous
Problem - incorrect base pairing.

listen to again and understand

Question 28

Endogenous threats of DNA

Answer 28

Endogenous – replication, transcription, ribose contamination, reaction with molecules in the cell such as water and oxygen

Question 29

Exogenous threats to DNA

Answer 29

Exogenous – reaction with molecules outside the cell, UV, cosmic rays, man-made chemical

Question 30

What can 8-oxoG pair with?

Answer 30

A or C

Question 31

Reaction of ROS with DNA chain

Answer 31

listen to and understand

Question 32

Act of transcription by itself generates breaks.

Answer 32

Demethylation which generates reactive oxygen species

R-loop formation – source of DNA breaks.

Question 33

Summary

Answer 33

Listen to summary answers

Question 34

Likely to be in exam so understand

Answer 34

During transcription activation you have demethylation of histones and DNA to remove 5’methyl group and 5’methyl cytosine. By product you generate lots of ROS. Mainly happens in non-coding regions, such as promotors and enhancers as you get lots of methylation events and you need to remove it in order to start gene expression.