Reverse Engineering Cells with CRISPR/Cas9 Genome-wide Screens Flashcards
Define
Co-dependent function
- Rescue, AKA resistance/masking/suppressors
- A mutation or defect in one gene is compensated for or alleviated by a second mutation in a different gene.
Define
Redundant function
- Synthetic sickness/lethality AKA sensitivity/enhancers/conditional essentiality
- Multiple genes or genetic elements perform overlapping or similar functions within a biological pathway or process.
Describe
The cell death - optimal growth spectrum
Synergy = interaction = redundancy = antagonism
Relationship between cellular processes associated with growth and those associated with cell death or apoptosis.
Describe
The ways to make a gene knock out/down in mammalian cells?
- RNA interference (knock down, low efficiency, many off-target effects)
- TALENs (engineered restriction enzymes)
- Gene-trapping
- CRISPR/Cas9
- Drug/compound
Define
CRISPR/Cas9
- Clustered Regularly Interspaced Short Palindromic Repeats
- Taken from a bacterial adaptive immune system
Define
Cas9
- CRISPR-associated protein 9
- Generates DNA DS break, guided by a 20-bp sgRNA 3 bases before PAM
What are the two strategies for large-scale gene KO phenotype screening?
- Arrayed
- Pooled library
What are the advantages and disadvantages of arrayed screening?
- More possible readouts and easy follow-up experiments
- Slow, expensive
- Requires robots
- Reliance on technical replicates
What are the advantages and disadvantages of pooled screening?
- Many readouts from one experiment; built-in biological replicates; can be run by a single biologist
- Fewer possible readouts, requires next-gen methods, need to maintain representation (enough cells)
What are the components of library design?
- Choose target regions (all coding regions)
- Generate all potential sgRNAs
- Choose 7-10 sgRNAs per gene (biological replicates)
- Minimize off-target effects
- Optimize on-target KO efficiency
How to optimize on-target KO efficiency?
- Optimize sequence (PWM or metling T)
- Avoid alternatively spliced exons
- Avoid the 3’ end where frameshifts could produce proteins
- Favor the coding “+” strand
PWM: By comparing a Position Weight Matrix with a DNA sequence, you can predict potential binding sites for transcription factors or other DNA-binding proteins
What does RANKS stand for?
- Robust Analytics and Normalization for Knockout Screens
What is the cell essentialome structured like?
- Structured like an onion
- Universal essential genes at the core of essential proteins complexes, as a dense cluster
What can chemogenomics reveal?
- Mapping pathways and gene functions
- Mechanisms of action/resistance
- Predict drug-drug synergism/antagonism
- Tumor-specific vulnerabilities
How are imperfect knockouts useful?
- Frameshifts near the end of the coding region can lead to a viable (hypermorphic?) protein
- In-frame mutations reveal amino acid-level fitness effects
- Heterozygotes can also be generated
