Health and Disease Dr Boyes

Question 0

What causes different genes to be expressed?

Answer 0

Transcription factors.

Question 1

Is DNA or genetic information lost during differentiation?

Answer 1

No

Question 2

What does tissue specific gene expression rely on?

Answer 2

A combination of the activity of specific transcription factors and chromatin modifications.

Question 3

What is Epigenetic regulation?

Answer 3

A change in state of expression of a gene which does not involve a mutation but is inherited, after cell division, in the absence of the signal, or event, that initiated the change.

Question 4

What determines which gene is activated?

Answer 4

The DNA binding domain on the transcription activators as they determine which promoter is activated.

Question 5

What determines rate of expression of a given gene?

Answer 5

Transcription factors and promoters, with the transcription initiation complex playing a role in the rate.

Question 6

Do promoters have multiple binding sites?

Answer 6

Yes, for various transcription factors.

Question 7

Describe how DNA is packaged?

Answer 7

In a nucleosome, wrapped around a histone octamer with a diad centre, then 10 nm fibre, then 30 nm fibre and the attached with loops to the protein scaffold.

Question 8

What are DNase 1 hypersensitive sites?

Answer 8

Found at promoters and enhancers of expressed gene, generated by the binding of transcription factors and the displacement of histone octamers. DNase 1 digests hypersensitive sites around 100x faster that other sites.

Question 9

How are DNase 1 sites mapped?

Answer 9

Cleave with DNase 1 in nuclei, prepare the DNA, cut with a specific restriction enzyme, electrophorese, Southern blot and probe with region next to the restriction site. The calculate the distance the hypersensitive site is from the restriction site.

Question 10

What has to occur before transcription?

Answer 10

Removal or relocation of the histone octamer at promoters by nucleosome remodelling complexes.

Question 11

What two mechanisms are there to remove or relocate the histone octamer at promoters?

Answer 11

Sliding histone octamers to new positions or displacement of the histone octamers.

Question 12

How does the nucleosome remodelling complex translocated the DNA around the nucleosome?

Answer 12

Using ATP taking 10 nm steps, coordinated by the DNA binding and translocation domains. The remodeller binds DNA in the linker and pushes it histone octamer to create a loop which passes through the translocation domain.
Push-me, pull-me idea.

Question 13

What are the other functions of the nucleosome remodelling complex?

Answer 13

Correct nucleosome spacing, DNA exposure, exchange of H2A/H2B dimers, CHD involved in repression.

Question 14

How can histone tails be modified?

Answer 14

Many sites, many acetylation via acetyltransferase co activators.

Question 15

What are changes in DNA methylation nearly always?

Answer 15

Inherited

Question 16

What are histone modifications?

Answer 16

Can be inherited and therefore Epigenetic. Eg. Polycomb H3K27me3 and Trithorax H3K9me3.

Question 17

What can Epigenetic changes cause?

Answer 17

The same transcription factor to activate different genes in different cell types.

Question 18

Where does CpG methylation occur?

Answer 18

On the cytokines of CpG dinucleotides and can occur at CNG in plants.

Question 19

What is required for the determination of genes being on or off?

Answer 19

Inherited Epigernetic mark and for it to do something for transcription.

Question 20

How are DNA methylation patterns inherited upon replication?

Answer 20

Newly synthesised daughter strands are hemi-methylated and converted to fully methylated state by Dntm1. The ‘perfect’ Epigenetic mark is maintained as somatic cells divide and the methylation is maintained by Dnmt1, required every time DNA is replicated, de novo methylation by Dnmt3 a and b.

Question 21

When does de novo methylation occur?

Answer 21

Only at high levels during embryonic development but can occur at low levels during different developmental stages.

Question 22

What does Dnmt stand for?

Answer 22

DNA methyl transferases.

Question 23

Describe Dnmt’s?

Answer 23

C-terminal highly conserved catalytic domain. Unconserved N-terminal domain.

Question 24

What does Dmnt3 a and b associate with?

Answer 24

Regulatory factor Dmnt3L.

Question 25

What are the two types of DNA demethylation?

Answer 25

Passive and active.

Question 26

Describe passive DNA demethylation?

Answer 26

One strand fails to be converted to the fully methylated form at replication and then becomes inherited in daughter cells via exclusion of the maintenance methyl transferase.

Question 27

Describe active DNA demethylation?

Answer 27

Methyl-cytosine is removed from DNA via enzymatic activity. This occurs much quicker and it’s important during embryonic development to re-set Epigenetic marks.

Question 28

What percentage of CpG dinucleotides are methylated?

Answer 28

70-80%

Question 29

What percentage of the mammalian genome is CG?

Answer 29

40%

Question 30

Why is methylation of CpG underestimated?

Answer 30

As 5-me-c is mutagenic and spontaneously deaminates. Methyl-cytosine deaminates to thymine, non-methyl-cytosine deaminates to uracil.

Question 31

What accounts for 50% off point mutations in genetic disorders?

Answer 31

5’-methyl-cytosine mutations which are not efficiently repaired.

Question 32

How are CpG dinucleotides distributed in a) invertebrates and b) vertebrates?

Answer 32

a) all of the genes are in unmethylated blocks.
b) methylation seems to have spread and there are small blocks without methylation which are found around gene promoters.

Question 33

What are small blocks in CpG dinucleotides without methylation called?

Answer 33

CpG Islands.

Question 34

Describe CpG Islands?

Answer 34

~1 kb long, GC rich, unmethylated in all (particularly germlines) tissues, at the promoter region of all housekeeping genes and 40% of tissue-specific genes, they span the promoter and into the first exon, some replication origins map to CpG Islands.

Question 35

What are the orphan CpG Islands often?

Answer 35

Sites of transcriptional initiation.

Question 36

What two methods are used to detect DNA methylation?

Answer 36

Restriction enzymes: use non-methyl specific to cut DNA when DNA sites are not methylated.
Bisulphite sequences: treat DNA with sodium sulphite which accelerates the deamination of un-methylated cytosine to uracil but it doesn’t affect the methylated cytosine.

Question 37

How does DNA methylation repress transcription directly?

Answer 37

Prevents transcription factors from binding.

Question 38

How does DNA methylation repress transcription?

Answer 38

Methylated DNA binding proteins bind to methylated CpG and prevent transcription factors from binding to promoters. This is more common.

Question 39

When can CpG Islands become methylated?

Answer 39

On the inactive X chromosome and in some cancers.

Question 40

What do methylated CpG Islands do?

Answer 40

Strongly repress transcription.

Question 41

What are the 3 classes of promoters?

Answer 41

CpG Islands, weak CpG islands, low CpG promoters.

Question 42

How do the three types of promoters vary?

Answer 42

CpG Islands: one CpG every 10 bp
Weak CpG Islands: one CpG every 20-30 bp
Low CpG promoters: one CpG every 100 bp.

Question 43

What is the methylated DNA binding protein MeCP1s activity equivalent to?

Answer 43

Kaiso and MBD2/HDAC

Question 44

What does the histone code hypothesis predict?

Answer 44

That modifications on the histone provide binding sites for chromatin-associated proteins and modifications on the same or different histone tails may be interdependent and generate various combinations on any one nucleosome. And this leads to the generation of active or repressed regions of chromatin.

Question 45

What does the histone code hypothesis imply?

Answer 45

That the chromatin structure of euchromatin or heterochromatic domains are dependent on the combination of differentials modified nucleosomes.

Question 46

What are the four key examples of histone modifications that lead to the binding of activators or repressors?

Answer 46

Acetylation of histone tails (activators bind via their bromodomains), tri-methylation of H3K4 (binding of activators via their PHD fingers), tri-methylation of H3K9 (binding of a repressor HP1 via its chromodomain), tri-methylation of H3K27 (binding of a repressor complex, polycomb repressor complex 1, via the chromodomain)

Question 47

During the formation of active or repressive chromatin what cooperates?

Answer 47

Chromatin marks and activator/repressor proteins to re-I force the activation/repression.

Question 48

What are the promoters and enhancers of active gene characterised by?

Answer 48

The presence of DNase 1 hypersensitive sites.

Question 49

What are DNase 1 hypersensitive sites?

Answer 49

Typically lack canonical nucleosome and are bound by a variety of transcription factors. Become activated from a repressed state via cooperation between nucleosome remodelling factors and histone acetyltransferases.

Question 50

What do nucleosome remodelling factors do?

Answer 50

Use the energy from free ATP to remodel nucleosomes at the hypersensitive site.

Question 51

What do histone acetyl transferases do?

Answer 51

Acetylate histone tails of nucleosomes in the vicinity of the promoter.

Question 52

Why are nucleosome remodelling complexes required?

Answer 52

To remodel the nucleosomes to allow for the pre-initiation complex to bind, for transcription to initiate. Specific upstream activators recruit them.

Question 53

What else is recruited to aid in activation?

Answer 53

Co-activators are recruited to facilitate activation from the factor to the pre-initiation complex.

Question 54

What do a number of the co-activators have?

Answer 54

Acetyltransferase activity, leading to acetylation of the nucleosomes in the vicinity of the promoter.

Question 55

What does the acetylation of the nucleosomes in the vicinity of the promoter provide?

Answer 55

Binding sites for proteins with bromodomains. This activating modification helps to recruit other chromatin activating proteins thereby reinforcing a it’s activity of this region of chromatin.

Question 56

What is a different activating chromatin mark?

Answer 56

The trimethylation of histone H3 at Lysine 4.

Question 57

What is the other activating chromatin mark mediated by?

Answer 57

SET1 and other related proteins.

Question 58

What recruits the mediator for the other activating chromatin mark?

Answer 58

The imitated form of the RNA pol 2, found only in the immediate vicinity of promoters (modification therefore found only on about 5 nucleosomes in the vicinity of the promoter).

Question 59

What are H3K4me3 often bound by?

Answer 59

Proteins with a PHD (plant homeodomain) finger. The binding of these helps to recruit other chromatin activating proteins thereby reinforcing activity of this region of chromatin.

Question 60

What is a common features of the two well characterised repressing chromatin marks?

Answer 60

These repressive marks are bound by repressors that then recruit enzymes that catalyse the addition of the repressive chromatin marks to adjacent nucleosomes. Thus, the presence of these modification helps to recruit other chromatin repressor proteins, thereby reinforcing repression of these regions of chromatin.

Question 61

What does the trimethylation of H3K9me3 provide?

Answer 61

Binding sites for heterochromatin protein 1, which binds via its chromodomain and them recruits methytransferase Suv39h which methylated adjacent nucleosomes via its SET domain. Facilitates the spread of heterochromatin.

Question 62

What does the trimethylation of H3K27me3 provide?

Answer 62

Binding sites for polycomb repressor complex 1, bonds via its chromodomain and recruits a second polycomb repressor complex 2 which includes Ezh2 which has methytransferase activity. Spread of the repressive mark through recruitment of the enzyme that catalyses addition of the histone mark.

Question 63

How do transcription factors bind to DNA?

Answer 63

The outside of the DNA double helix can be read by proteins. Recognise helix-turn-helix motifs, zinc finger domains, leucine zippers, basic helix-loop-helix.

Question 64

How do proteins bind DNA?

Answer 64

Bind in the major groove by hydrogen, electrostatic and hydrophobic interactions, typically 10-20 contacts. Contribute to strength and specificity. More information is present in major groove compared to minor and consequently more proteins bind here.

Question 65

What is the helix-turn-helix motif?

Answer 65

N-terminal structural helix with a turn and a c-terminal recognition helix.

Question 66

How do helix-turn-helix motifs bind DNA?

Answer 66

In the major groove, usually as dimers.

Question 67

What are the two types of zinc fingers?

Answer 67

2 cysteine- 2 cysteine and 2 cysteine- 2 histidine

Question 68

Describe 2 cysteine- 2 cysteine zinc fingers?

Answer 68

Bind as dimers with four zinc fingers, the two halves of the recognition site are separated by one turn of the DNA helix. The n-terminal finger is involved in DNA binding and the second fingers determines the optimal spacing between the two halves of the palindromic recognition site. Best example is DNA binding domain in nuclear hormone receptors.

Question 69

Describe 2 cysteine- 2 histidine zinc fingers?

Answer 69

Has an antiparallel beta sheet leading into an alpha helix, the zinc coordinates four amino acids to hold one end of the alpha helix and one end of the beta sheet. Can have a number of zinc fingers which allows of almost continuous stretch of alpha helices that can form contacts.

Question 70

Describe zinc fingers?

Answer 70

Used to coordinate and structure the DNA contacts, each recognises three bp.

Question 71

Describe leucine zippers?

Answer 71

Bind as dimers with alpha helices contacting the DNA sequences in the major groove. Leucine is repeated every 7 amino acids and therefore allows dimerisation via hydrophobic interactions. Grips like a clothes peg.

Question 72

What can heterodimerisation of leucine zippers do?

Answer 72

Can alter the DNA binding specificity.

Question 73

Describe the basic helix-loop-helix?

Answer 73

Short helix mediates dimerisation and the loop and long helix mediates DNA binding. Flexibility of the loop allows odd the helices to pack against eachother.

Question 74

How can basic helix-loop-helix be inactivated?

Answer 74

By dimerisation with partners that lack DNA binding domains as dimerisation regulates DNA binding.

Question 75

Give the two types of designer transcription factors?

Answer 75

Zinc finger nuclease and TALE system.

Question 76

What are zinc fingers used for and what are their disadvantages?

Answer 76

Can be hooked to Fok1 endonucleases to introduce breaks at specific sites in the genome.
Disadvantages: must bind palindromic DNA sequences as a dimer, each finger recognises a triplet of bp and not all are recognised specifically.

Question 77

What are TALE systems?

Answer 77

Designer transcription factor newly developed for Xanthomonas. Can build up proteins that bind any sequence of choice. A 34 amino acid repeat where 12 and 13 recognise the specific base. They build-up seigneur DNA binding proteins by linking these individual repeats in the correct order.

Question 78

How do transcription factors work?

Answer 78

They stimulate activity of the basal promoter complex. Can use multiple mechanisms to provide synergistic activation.

Question 79

What are the mechanisms by which transcription factors work?

Answer 79

Using activation domains that contact different TAFs in the TF2D complex, activators can functions via TF2B to alter the configurations of the basal machinery to enable it to recruit components more efficiently or to enhance he rate of binding of TF2B, activators can interact with the mediator complex, activators can recruit co-activators/repressors to contact basal machinery or to open the chromatin.

Question 80

How can genes be regulated?

Answer 80

By the presence or absence of a transcription factor or by converting a transcription factor between inactive and active states.

Question 81

What are the advantages of regulation by transcription factors activations?

Answer 81

Allows a rapid response, allows regulation on response to external factors, frequently used by signalling pathways, allows fine tuning of transcription level.

Question 82

How can transcription factors be activated?

Answer 82

By binding to a ligand, by protein modifications (phosphorylation, acetylation and ubiquitination), by cleavage of larger precursors, by dissociation of an inhibitor protein.

Question 83

How does binding of ligand activate transcription factors?

Answer 83

Induces a conformational change in nuclear hormone receptors, triggering DNA binding and gene activation. Also permits interaction with co-activators such as CBP, SRC-1 and SRC-3.

Question 84

Why is phosphorylation modification often used to activate transcription factors?

Answer 84

In response to cell surface receptor signalling.

Question 85

What does activation of TF by phosphorylation do?

Answer 85

Allows cells to respond to the environment by increasing protein activation, interaction with other proteins and co-activators.

Question 86

What is the most simple method of phosphorylation?

Answer 86

Direct phosphorylation by cell surface receptors. Cytokines activate JAK/STAT pathway.
Cell surface receptors transmit the signal to JAKs that phosphorylate STAT transcription factors. This causes dimerisation of STATs and translocation into the nucleus where they bind specific target genes.

Question 87

What is a more complex method of activation of TF by phosphorylation?

Answer 87

Binding of ligands to receptor tyrosine kinases activates the Ras/raf/MAPK kinase cascade. Signalling cascade allows amplification of signal growth factors bind receptor tyrosine kinases. This triggers autophosphorylation and activation of Ras. Ras binds GTP activating it. This phosphorylates Raf which phosphorylates other kinases in the pathway.

Question 88

What does phosphorylation of TF do?

Answer 88

Allows a transcriptional change based on growth/environmental signals.

Question 89

What does acetylation do?

Answer 89

Increases TF binding to DNA, increases protein interactions and has positive or negative effects on protein stability.

Question 90

How is acetylation typically added?

Answer 90

By histone acetyltransferases (HATs) co-activators bound to promoters.

Question 91

What does acetylation of GATA-1 do?

Answer 91

Increased GATA-1/DNA binding.

Look into if you have time.

Question 92

What are the properties of GATA-1 acetylation?

Answer 92

Stimulates GATA-1/DNA binding and GATA-1 dependent transcription, enhances GATA-1/protein interactions, is required for proper GATA-1 function during haematopoietic differentiation, modulates GATA-1 levels.

Question 93

How does Ubiquitination TF activation generally occur?

Answer 93

Triggered by other protein modifications, usually phosphorylation.

Question 94

What does poly-ubiquitination cause?

Answer 94

Protein degradation.

Question 95

What is Ubiquitination?

Answer 95

Requires E1, 2 and 3 ubiquitin Ligases to add ubiquitin.

Look into more if you have time.

Question 96

How is TF degradation and pol2 transcription linked?

Answer 96

The activator interacts with basal transcription machinery recruiting ubiquitin Ligases that modify the transcription factors. This Ubiquitination recruits the 26S proteasome simultaneously destroying the activator and promotes pol 2 elongation.

Question 97

How does TF degradation linked to pol2 transcription limit uncontrolled transcription?

Answer 97

By destroying the activator each time the promoter fires and by ensuring that it’s activator is at a promoter that are destroyed by the proteasome.

Question 98

When is activation of TF by cleavage of larger precursors important?

Answer 98

During neuronal development.

Question 99

Give the three long-range control elements?

Answer 99

Enhancers, LCRs and insulators.

Question 100

Describe enhancers?

Answer 100

Long range, from 1 to 1000 kb from the gene controlled, positive control elements, may be up several kb from promoters and contain multiple transcription factor binding sites.

Question 101

Describe LCRs?

Answer 101

Very strong enhancers, gives position-independent copy number dependent expression of the transgene, discovered as essential elements to generate transgenic mice, either 5’ or 3’ of the gene, often found as string DNase 1 hypersensitive sites, bound by many tissue-specific transcription activators.

Question 102

Describe insulators?

Answer 102

Long range, prevent interference by regulatory elements in neighbouring genes, block enhancers from interacting with the promoter, second function is to block the spread of heterochromatin.

Question 103

Why is it beneficial to block the spread of heterochromatin?

Answer 103

Barrier function: important to protect genes from silencing.

Question 104

How was the barrier function assayed?

Answer 104

Using stable transfection reporter constructs.

Question 105

What occurs in the absence of an insulator?

Answer 105

The reporter gene becomes repressed followed by heterochromatin formation.

Question 106

What can reporter constructs be used for and why is this beneficial?

Answer 106

To assay the regulation of gene expression.

Rapid, quantitative assay and can use the same assay to quantify expression of different constructs.

Question 107

How can transfection into cells differ?

Answer 107

Can be transient or stable, can be into cell lines of type where genes are normally expressed, can be into heterologous cell lines together with co-transfection of an expression vector.

Question 108

How are transgenic mice generated?

Answer 108

The transgene is injected into he male pronucleus of one cells embryo. Forster mothers are made pseudopregnant by mating with a vasectomised male.

Question 109

How is the transgene inserted into the genome?

Answer 109

Randomly, head-to-tail manner. DNA is isolated from the vector backbone prior to injection of the transgene.

Question 110

What vectors can be used to generate transgenic mice?

Answer 110

Plasmid- insert up to 20 kb 
Cosmid- insert up to 45 kb 
BAC- inserts 100-300 kb (look into more if you have time) 
YAC- inserts up to 1 Mb
Initial analyses of LCRs-mini locus

Question 111

Explain how promoters can be linked to reporter genes to more easily analyse expression?

Answer 111

Location of lacZ expression can be determined by fixing the embryos and then reacting them with X-gal. This enables the location of expression of the gene in the embryo to be readily determined. Promoter deletions and mutations can also be made to determine what regulates gene expression at distinct stages of development.

Question 112

What are the advantages of analysing gene expression in transgenic mice?

Answer 112

In vivo: transgene is exposed to factors at correct stages of development. Reporter genes can be used to analyse when promoters are activated during development.

Question 113

What are the disadvantages of analysing gene expression in transgenic mice?

Answer 113

Copy number is different from line to line, insertion site is random (insertional mutagenesis) position effects, need to analyse many transgenic lines to ensure that the effects are real.

Question 114

How can you overcome some position effects?

Answer 114

Use LCRs and insulators.

Question 115

How does generation of knock-in mice differ from he generation of knock-out mice?

Answer 115

Same but knock-out mice delete whole genes, regions of genes or gene regulatory elements and knock-in mice mutate regions of a gene of mutate specific regions of the gene regulatory elements. Substitution rather than deletions.

Question 116

What are the disadvantages with knock-out mice?

Answer 116

15% are embryonic lethal, some knock-outs show no effects (compensated by closely related gene product), if the genes work in combination with other genes the effects are not always fully apparent in all organs.

Question 117

How can conditional knock-out mic be made?

Answer 117

By flanking with LoxP sites, placing of the LoxP sites allows a number of different conditional rearrangements, look into more if you have more time.

Question 118

What can Cre recombinant be used for?

Answer 118

To inactivate or activate gene expression, inducible cause changes in gene expression. Tissue-specific expression of Cre causes changes in the target heme only in those tissues, inducible Cre allows target gene inactivation at a controlled time.

Question 119

Conclude how enchanters work?

Answer 119

Physically touch promoters, consistent with looping hypothesis. On come cases there is evidence that the enhancers reach promoters via facilitated tracking. However, it is currently unclear at how many promoters facilitated tracking will play a role.

Question 120

What is essential for the enhancer blocking function of insulators?

Answer 120

CTCF an 11 zinc finger protein that can either activate or repress transcription.

Question 121

What properties allow CTCF to have its enhancer-blocking function?

Answer 121

Interaction with cohesion and association with the nuclear lamina.

Question 122

Conclude how insulators work?

Answer 122

Increasing evidence that insulators work by forming chromosome loops that prevent the enhancer from interacting with the wrong promoter. Insulators potentially also function by blocking tracking of the enhancer.