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Lecture notes BIOL3015 Epigenetics $7.11   Add to cart

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Lecture notes BIOL3015 Epigenetics

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Lecture notes from a series of lectures in BIOL3015 Regulation of Gene Expression, epigenetics. Covering: DNA methylation, chromatin structure, epigenetic modifiers, non-coding RNAs, Epigenetics and disease, social environment, cancer and tumour supression

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  • December 11, 2023
  • 13
  • 2021/2022
  • Class notes
  • Karen lillycrop
  • Biol3015 epigenetics
  • Unknown
  • Unknown
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Epigenetics
Epigenetics
 Literally means ‘on top of genetics ‘
 Definition – Processes that include long-term stable changes in gene activity without
a change in gene sequence
 Main 3 processes are: DNA methylation, Histone modification and non-coding RNAs

DNA methylation
 Cytosine is methylated to 5-methyl Cytosine
 90% of methylated cytosine is found as a dinucleotide CpG
 Hemi methylated – one strand methylated
Mapping methylation status of genes
 Two restriction enzymes used:
 MspI – recgonises and cuts CCGG, will also cut CCMeGG
 HpaII – only cuts CCGG is second C is not methylated
 If 3 unmethylated CCGG both enzymes will cut all of them
 If a site is methylated, Msp1 will cut all sites, Hpa2 will only cut non methylated
CCGG
 Hence, different size bands are left
 Can show if methylation is present
Analysis of methylation status of the globin gene
 Erythroid cells produced the same number of bands of the same size hence no
methylation
 Liver cells Msp1 got two bands whereas Hpa2 only had one band
 If the gene transcriptionally active then the cells were unmethylated (Erythroid), but
if the gene transcriptionally inactive then the cells are methylated (Liver cells)
Methylation and transcription
 If low levels of methylation in the promotor region – the gene active
 high levels of methylation in promotor regions – gene inactive
Model for DNA methylation inhibition of gene expression
 Transcription factor binding is blocked by DNA methylation
 MeCP2 (Methyl CpG binding protein) Binds to methylated CpG and coats it to block
RNA polymerase
DNA methyl transferases (DNMTs)
 DNMT 1:
 Copies methylation marks from original strand of DNA onto new DNA
 DNMT3a and 3b: de novo DNMT’s:
 Responsible for establishing methylation marks
 If removed in mice – they are lethal
 DNMT2 not lethal in mice – unknown function
Search for DNA demethylase
 Could not be found
 Suggested that passive process could remove methylation
 Dnmt1 does not replicate methylation marks, leaving hemimethylated DNA which in
the next round of replication will produce DNA without methylation
Active demethylation

,  Hydroxy methyl cytosine (hmC)
 Found in 1972
 2009 Tet1 (ten-eleven translocase 1) found to convert 5mC to 5hmC)
 Hydroxy form is thought to be intermediate in demethylation of DNA
 Oxidation or deamination can then remove methylation
5hmC an intermediate in removal of 5mC
 Low levels in the genome (less than 105 of 5mC i.e., short-lived entity)
 Over expression of tet1 leads to decrease in 5mC, increase in unmethylated Cytosine
 Tet 1 depletion leads to an increase in 5mC

Chromatin structure
 Nucleosome structure
 DNA loop wrapped around a core of histones
 Histones are positively charged proteins – 8 histones
 Nucleosome is then folded upon itself to make a solenoid structure/ 30nm fibre
 Further looped and compacted to form 200 nm fibre which forms DNA in cells
DNase 1
 Endonuclease that cleaves double-stranded DNA
 Chromatin from erythroid cells added to increasing concentration of DNase 1
 Run on gel, blot and hybridized with probes from gene of interest
 Ovelbumin – transcriptionally inactive in cells – little or no digestion of gene –
condensed form so difficult for DNase 1 or RNA polymerase to access
 globin gene – Active in cells – complete digestion of gene even in low
concentrations – easy for DNase 1 and RNA pol to gain access
Chromatin structure
 Loose or tight
 Transcriptionally active gene – unmethylated – relaxed structure – accessible to RNA
pol
 Transcriptionally inactive – methylated – condensed structure – not accessible to
RNA pol
DNase 1 hypersensitive sites
 Erythroid cells –




 Located at the 5 prime ends of genes
 Are nucleosome free
 Initiation is reduced on DNA that is associated with nucleosomes
Transcription factors can recruit co-activators
 Modify histone structure

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