PCR

Question 1

What does PCR do?

Answer 1

Amplify a sample of DNA.

Question 2

What is required for PCR? List 4 components.

Answer 2

1. Primers
2. dNTPs (nucleotides)
3. Template ssDNA
4. Taq polymerase

Question 3

Why is Taq polymerase used?

Answer 3

It is thermostable and high temperatures are needed.

Question 4

What happens to the amount of target ssDNA with each round of PCR (theoretically)?

Answer 4

It doubles.

Question 5

What are the 3 main steps in a PCR cycle?

Answer 5

1. Denature the DNA by heating to 95 degrees.
2. Cool the mixture to between 45-72 degrees to allow annealing of the primers.
3. Heat the mixture to 72 degrees to allow the polymerase to work.

Question 6

Which region does PCR selectively amplify?

Answer 6

The region between the primers.

Question 7

What happens to the DNA fragments over successive rounds?

Answer 7

They become closer in length to the distance between the 2 primers.

Question 8

What are the 4 main sources of error in PCR?

Answer 8

1. Contamination - it is a v. sensitive process, contaminants are amplified along with the DNA.
2. Innappropriate priming - primers that are not 100% accurate can still bind, especially if the 3’ end of the primer matches the DNA.
3. Taq polymerase is highly error prone.
4. GC rich areas of DNA are hard to amplify.

Question 9

PCR can be used to introduce ‘site-directed mutagenesis’. What does this mean?

Answer 9

It can introduce specific changes into the DNA sequence for genetic engineering.