Lecture 2 - CRISPR II Flashcards
Define Interference
Process of Surveillance, Targeting and Degradation of MGE DNA
(i) How is crRNA processed and loaded into interference complexes
(ii) How does crRNA mediate interference?
(i) CRISPR loci is transcribed to RNA (pre-crRNA), which is processed and loaded into interference proteins
* crRNA - produced from single DNA spacer
(ii) crRNA in interference protein complexes base-pairs with complementary MGE DNA, targeting nucleolytic activity of interference complex to specific sequences
Compare the interference complexes produced for Class I and Class II CRISPR Systems
Class I - multiprotein surveillance complex (cascade), which recruits nuclease-helicase Cas3 to cleave MGE
Class II - single protein complex, which may require tracrRNA for assembly (signals Cas9 to fold/activate)
(i) How is the R-loop formation triggered/ activated?
(ii) What is this known as?
(3 Points, 1 Point)
(i) R-loop formation is triggered by two factors:
* Detection of PAM sequence
* Formation of seed region (locks R-loop in place)
(ii) Known as Surveillance Events of Interference
How is the R-loop involved in the interference process?
R-loop formation recruits effector proteins (e.g., Cas3 - recognises ssDNA) that cleave up the MGE DNA
Define the two major functions of Interference Protein Complexes
- Surveillance for complementary MGEs
- DNA cleavage to destroy recognised MGEs
(i) What is the Seed Region?
(ii) Why is Seed Formation important?
(i) 6-8nt upstream of PAM sequence which must be complementary to the target for recognition
* provides specificity
(ii) Seed Formation (i.e. Base Pairing) - provides sufficient energy for “snapping/locking” onto DNA, forming the R-loop structure
(i) What is the Function of the Protospacer Adjacent Motif (PAM)?
(ii) How do they functionally couple adaptation and interference?
(i) Marks site of protospacer sequence for interference complex, but is not integrated into CRISPR Loci to prevent self-recognition
(ii) Involved in both Interference and Adaptation
What is the CasA/Cse1 subunit?
Component of cascade interference complex that recognises PAM
(i) How does the CasA subunit recognise the PAM?
(ii) Why is this significant?
(i) PAM sequence (e.g., ATG) is recognised in double strand form via its minor groove (H-bond patterns)
(ii) This recognition method allows some mismatched PAMs to be tolerated, providing target strand sequence is optimal
Define Cas3 in terms of:
(i) Structure + active site composition
(ii) Recruitment
(iii) Function
(i) Multidomain Polypeptide, containing HD domain in active site (Catalytic Histidine/Aspartate residues)
(ii) Recruited to Interference complex via ssDNA
(iii) ATP-dependent Translocase/Nuclease, moving along ssDNA and cleaving it into fragments
Describe the Structure/Assembly of the Cas9 Interference complex
crRNA base-pairs with tracrRNA, which forms a scaffold that recruits/loads onto the Cas9 effector protein
What are the two major functions of tracrRNA?
- Cutting pre-crRNA into crRNA, comprising of a single spacer sequence (by RNase III)
- Activation of Cas9 apoenzyme into haloenzyme/ nuclease enzyme
Describe the structures of the two Cas9 Nuclease active sites
- RuvC-like - based upon Aspartate residues
- HNH/RNase-like - based on a Histidine residue
How can Cas9 be used for genome editing?
(2 Points)
- Cas9 nuclease activity can be utilised to induce double-strand breaks at specific sites within the genome (due to crRNA/gRNA)
- dsDNA breaks activate DNA repair mechanisms, which can lead to gene KO, mutational insertion or repair of mutated genes
