Test 3 CRISPR/Cas Flashcards

1
Q

Describe how the CRISPR/Cas system works in bacteria?

A
  • Foreign DNA acquisition
    • Viral DNA is cleaved and added to CRISPR array.
    • Transcription of locus
  • CRISPR RNA processing
    • CRISPR RNA is cleaved into gRNAs by nuclease.
    • The nuclease must be complexed with tracrRNA.
  • RNA-guided targeting of viral element.
  • Inactive Cas9 nuclease binds to gRNA and tracrRNA and becomes activated.
    • Recognizes a complementary target sequence and cleaves it.
  • RESULT: Recombination or Deletion.
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2
Q

Why is Cas9 inactive until it binds to gRNA and tracrRNA complex?

A

If it was activated it could spontaneously react to any DNA nearby.

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3
Q

Two types of nuclease-induced genome editing.

A
  • Homology directed repair:
    • Harder to do but fewer errors
  • Non-homologous end joining
    • Extremely error prone.
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4
Q

Describe the CRISPR/Cas system?

A
  • CRISPR array:
    • Protospacers and short repeats
  • Pre-crRNA is then joined with RNase 3, tracrRNA, and Cas9
  • The complex cleaves the crRNAs
  • The complex then looks for a target sequence (protospacer) which must be adjacent to a PAM (Protospacer adjacent motif).
  • The complex then binds downstream (3’ ) of PAM sequence
  • Cleaves both strands upstream of PAM
  • Then the complex unbinds.
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5
Q

Are tracrRNA and gRNA comined into one in the Lab?

A

YEA

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6
Q

2 components needed for Lab based CRISPR/Cas9

A

Guide RNA (gRNA) - contains both tracrRNA and gRNA

Cas9 nuclease

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7
Q

Explain the PAM sequence

A
  • Specific for each bacterial species
  • Found directly downstream of the target.
  • Required for Cas9 to work.
    • Cas9 partially unwinds the the DNA.
  • Thought to be present in every gene.
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8
Q

Requirements of CRISPR/Cas in a lab

A
  • The sequence is unique compared to the rest of the genome.
  • The target is present immediately upstream of a PAM
    • PAM sequence is NGG.
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9
Q

What does homology directed repair require?

A

A template

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10
Q

Explain Cas9 nuclease

A
  • Two endonuclease activities are present in a complex.
    • This means you can inhibit one and then selectively nick a single strand.
      • Using two different Cas9 complexes each with one domain inhibited. You can make a large change to the genome by cutting only one strand a distance apart. Then using a template (homologous directed repair) to splice it in.
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11
Q

Doubly inhibited Cas9 can be used for what?

A

To hold a transcriptional activator or repressor to activate or repress a target gene.

Hold GFP to ID a specific segment of the chromosome.

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12
Q

How can catalytically dead Cas9 be used?

A
  • Neutered Cas9 can be used to activate or inactivate transcription of histones
    • By binding a methylase to the complex DNA can be methylated using Cas9.
      • Methylation decreases gene expression
    • Demethylase can also be used.
      • Demethyation increases gene expression.
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13
Q

Limits of CRISPR/Cas in area of effect?

A
  • Germline cells can be modded to effect whole animal.
  • Somatic cells can be modded to effeect specific cells or tissues.
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14
Q

Application of CRISPR to treat cancer

A
  • IF an activated protein is causing cancer you could code a stop codon before the protein, and add the DNA back into the patient.
    • This would knock out the mutated protein.
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15
Q

Uses of CRISPR in the clinic

A
  • Precision therapy
    • Must ensure gRNA cant also bind elsewhere or there will be unintended side effects.
  • Disease modeling
  • Drug screening
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16
Q
A