CRISPR
CRISPR
CRISPR
Kiran Mishra
009
Sem 3
Msc Part II
Overview
01 Introduction
02 Altering PAM specificity
03 Enhancing Delivery systems
1960s 1990
Discovery of double helix Generation of first rDNA
Experiments
molecule
demonstrating role of
CRISPR Cas 9 together
Genome editing
the 9
Cas9
systems 02
activity
Increasing
03 uniformity of
edited cells
- SpCas9 recognizes the 5′-NGG-3′ PAM
SpGCas9
NGH PAM Sites PAM Sequence No. of sites tested Editing Efficiency
NGA 3 41.0–76.7%
NGT 3 35.7–83.7%
NGC 3 17.3–40.67%
N – A/C/G/T SpRY
Problem with plasmids – no • Disadv - small cargo size, thus the Cas systems and sgRNA
targeted delivery, poor control must be encoded on separate vectors
over Cas9.
Enhancing
delivery
systems
Lipid Nanoparticles
Ideal traits of delivery
• Cationic ionizable lipids - effective nucleic acid
methods –
encapsulation, cellular transport, and endosomal release.
• High editing efficiency • Light triggered Liposome – Verteporfin (photosensitive)
• Low immunogenicity
• Targeted delivery
Increasing uniformity of edited cells
- Hei tags for short
- Delivers Cas9 directly to the
nucleus
High Efficiency - hei-tag, a myc-tag coupled to
Tags an optimized NLS via a flexible
linker, to Cas9
- heiCas9 displayed a 70%
increase in bi-allelic targeting
efficiency
- Difference between HDR and NHEJ - Done in zebrafish as well, 17
pathways wrt to CRISPR editing . fold more results
- CtIP protein
- Addition of small N terminal of CtIP to
Cas9 Stimulating HDR
- Limitation – guides play some instead of NHEJ
unidentified role, therefore larger pool
of guides need to be tested to enhance
the efficiency to max.
Conclusion:
- CRISPR remains one of the best genome
editing tools.
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Thank You