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Epigenetics and Gene Editing (RUG) Complete Summary

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Complete and clearly structured summary of the course Epigenetics and Gene Editing (RUG). This document covers the key concepts of epigenetic regulation and modern gene editing technologies, linking chromatin and DNA-level mechanisms to gene expression control. It explains major epigenetic marks and how they are established and interpreted, as well as the principles behind CRISPR-based editing, DNA repair pathways, editing outcomes, delivery strategies, limitations such as off-target effects, and relevant ethical considerations. Written for efficient revision and exam preparation, with a clear structure and concise explanations. Includes • Full coverage of the main course topics • Clear structure and concise explanations to support fast studying • 44 pages in total for a complete overview

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Tijmen Lourens Summary Epigenetics and Gene Editing



Epigenetics and Gene Editing

Lecture 1

Epigenetics:
- Heritable, yet reversible changes in genome functioning, not encoded in the DNA
sequence
-

Induced Pluripotent Stem Cells: iPSCs: cell from human can be reprogrammed to stem cell
state.


Centromere: keeping the two chromatids together during mitosis.

Interphase is the most common phase, here the DNA is packed in
nucleosomes. During Mitosis (M-phase) the DNA is fully condensed.


Organization of chromatin:
- Interphase chromatin: fibers, roughly two types:
o Heterochromatin → very dense
o Euchromatin → more loose
- Tail of histone H3 is heavily subjected in post-translational
modification
o For all histones the tail sticks out
- Dimer of histones is formed between two different types of
histones, then these two bind again to form tetramer.

Nucleosomal DNA:
- No particular sequence, affected by DNA binding protein
- Tight association DNA-histones
- Breathing Is unregulated, protein is
regulated
o This breathing happens really short
and makes the DNA accessible for a
short period of time.


Chromatin remodelling:
- ATP dependent (controlled)
- Need to be recruited, need to know what to
do
o Nucleosome sliding makes sure some
parts become accessible / inaccessible

,Tijmen Lourens Summary Epigenetics and Gene Editing

Chromatin compaction: linker histone H1
- 1 molecule present per nucleosome core
- Binds DNA and protein
- Larger than other (individual) core histones
o Determines direction ‘nucleosome-outgoing’ DNA
- Histone 1 plays a role in compaction in bead on string configuration
- Tentacles seek contact with each other in order to come closer
o Can cause DNA around complex to get closer or farther away

Conclude this part:
- DNA is organized in nucleosomes
- Nucleosomes form chromatin fibers
- Chromatin compaction differences
o (euchromatin <-> heterochromatin (condensed))
- Chromatin is dynamic (+/- ATP):
o remodeling influences accessibility DNA
- Next:
→ chromatin types can be passed on to next generation of cells
→ Þ chromatin types associate with gene expression levels




EXAM! Very important to realise: 40% = fast majority (euchromatin) of DNA is open but not
actively expressed.
Also:
- Facultative heterochromatin: regulated if it is active/inactive
- Constitutive heterochromatin: permanent inactive

,Tijmen Lourens Summary Epigenetics and Gene Editing

Heterochromatin structure spreading:
- Position effect: active gene translocated to heterochromatin area → inactive
(silencing)
- Barrier: chromatin likes to spread until it comes across a barrier
o If there is no barrier between hetero- and euchromatin after translocation --.
Spreading of heterochromatin




Heterochromatin spreading and maintenance:
position effect variegation (PEV)
Variegation = “to make varied in appearance”
different appearance within one tissue
- White gene active = red pigment
- White gene inactivated = white spots




Acetylation: removing positive charge results in more ‘open’ chromatin structure →
expression activation (DNA is negatively charged)

Phosphorylation: introduces negative charge = ‘open’ chromatin structure → loosening up
its compaction by making the compound less positive!!!

Mutually excluded: if there is one modification the other one does not fit. (if a lysin is
acetyled it cannot be methylated also)

Methylation does not mean silencing directly, it can also associated with activation →
different tags recruiting proteins

, Tijmen Lourens Summary Epigenetics and Gene Editing

Summary:
- DNA in nucleosomes
o Packaging
o Controlling accessibility
- Nucleosomes exist in different forms:
o Histone modification (writers/erasers)
o Histone variants
- Different chromatin types: dynamic
o Eu-versus heterochromatin (chromatin
remodellers)
o Spreading, maintenance, transcription

Histone acetylation (in contrast to methylation) is always
associated with active gene expression.

Reader-writer complex binds to DNA sequence → reader-writer
complex spreads heterochromatin-specific histone tail
modifications and heterochromatin-specific protein bind →
heterochromatin spreads until it encounters a barrier DNA
sequence
- Reader-writer mitigates the process of heterochromatin
spreading over Reader Complex
- Reader-eraser protein binds and removes
heterochromatin-specific marks
- Erasers can also erase activating modifications to induce
silencing

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Material required for this course at the university of groningen.
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