Manipulation of Gene Expression Flashcards

1
Q

Why would we want to manipulate gene expression?

A

To investigate the biological function of a gene
To create cell/animal models of disease
For gene therapy

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2
Q

How can we study gene down-regulation?

A

‘Knock down’ gene expression
Look for a change in phenotype
Loss of function (LOF)

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3
Q

What is the ‘gold standard’ for investigation gene function?

A

Gene down-regulation

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4
Q

How can we study gene up-regulation?

A

‘Overexpression’ of a gene

Look for a change in phenotype

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5
Q

How would you achieve stable overexpression of a gene?

A

By the insertion of an extra copy of the gene of interest into the genome

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6
Q

What is a common way of delivery of extra copies of genes for stable overexpression?

A

Viral delivery, e.g. retroviral and lentiviral

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7
Q

How can we get constitutive expression of a inserted gene?

A

Put it under the control of a constitutive promoter

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8
Q

What are the disadvantages of gene insertion for stable overexpression?

A

The insertion of the gene may disrupt another gene
Is the effect caused by overexpression or by integration
Higher biosafety level than transient methods

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9
Q

What is a very widely used approach for gene knockdown?

A

RNAi

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10
Q

What does RNAi achieve?

A

Post-transcriptional gene silencing

Degradation of mRNA

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11
Q

What does RNAi utilise?

A

A natural anti-viral mechanisms found within most cells

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12
Q

What are the pros of using RNAi for gene knockdown?

A

Relatively cheap
Can be used both for transient and stable knockdown
Commercial pre-designed siRNA readily available
Targeting of specific splice variants possible

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13
Q

What are the cons of using RNAi for gene knockdown?

A

Off target effects are increasingly being reported

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14
Q

What are transcription like-activator effectors (TALEs)?

A

Synthetic transcription factor binding domains

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15
Q

What is the role of TALEs?

A

They are programmed to recognise specific DNA motifs

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16
Q

What are the pros of using TALEs?

A

Two TALEs required for FokI dimerisation

Very specific… fewer off-target effects than TALEs

17
Q

What are the cons of using TALEs?

A

TALEs need to be designed which is expensive and time consuming
They don’t always work

18
Q

What does CRISPR stand for?

A

Clustered regularly interspaced short palindromic repeats

19
Q

What is the CRISPR system?

A

A system found in bacteria to confer resistance to viral infection

20
Q

What is the protein associated with the CRISPR system and what does it do?

A

CRISPR-associated protein 9 (Cas9)

It is a nuclease that acts as a monomer to cause double strand breaks

21
Q

Does the CRISPR system temporarily or permanently modify DNA?

A

It is a permanent modification

22
Q

What is CRISPRi?

A

CRISPR interference
Also, commonly used to refer to CRISPR inhibition
It is reversible

23
Q

What is CRISPRa?

A

Activation of transcription

It is reversible

24
Q

Is RNAi an old or new technique?

A

Older technique but still widely used

25
Q

What are the pros of using RNAi?

A
Time efficient (shortest time to phenotype)
Highest level of off-target effects
Can target specific splice variants
26
Q

What are the pros and cons of TALEN?

A

More specific but is more difficult

27
Q

The CRISPR/Cas9 system has become very popular, why?

A

Because it is cheaper and easier than TALEN

28
Q

What are some of the considerations when trying to manipulate gene expression?

A

Short or long term knockdown to generate effect
Cell type: where is the gene expressed, use a primary or immortalised (cancer) cell line
Cell or animal model