D1.1.4 Polymerase chain reaction and gel electrophoresis

Question 1

What temperature is the denaturation step in PCR?

Answer 1

95°C.

Question 2

What happens during the annealing step?

Answer 2

The temperature is lowered to allow primers to bind to their complementary sequences on the single-stranded DNA.

Question 3

List the key components of PCR.

Answer 3

1. Template DNA
2. Primers
3. Taq polymerase
4. Nucleotides (dNTPs)
5. Thermal cycler.

Question 4

What is the temperature range for the annealing step in PCR?

Answer 4

50-65°C.

Question 5

What is the role of the buffer solution in gel electrophoresis?

Answer 5

It conducts electricity and maintains a stable pH during the electrophoresis process.

Question 6

What happens to DNA in the gel during electrophoresis?

Answer 6

DNA, being negatively charged, moves toward the positive electrode.

Question 7

What is the gel in gel electrophoresis made of?

Answer 7

Usually made of agarose.

Question 8

What is gel electrophoresis?

Answer 8

A technique used to separate and analyze molecules like DNA based on their size, charge, or shape.

Question 9

Why is Taq polymerase used in PCR?

Answer 9

Because it is heat-resistant and remains stable at high temperatures.

Question 10

How many times is the PCR cycle typically repeated?

Answer 10

20-40 times.

Question 11

What happens during the extension step?

Answer 11

Taq polymerase adds nucleotides to the primers, synthesizing new DNA strands.

Question 12

What is the first step in the gel electrophoresis process?

Answer 12

Preparation of the gel, usually made of agarose.

Question 13

What happens during the denaturation step?

Answer 13

The DNA double helix is heated to 95°C, breaking the hydrogen bonds and resulting in two single strands.

Question 14

What happens to the gel after electrophoresis?

Answer 14

The gel is stained with a dye that binds to DNA, making the fragments visible under UV light.

Question 15

What is the purpose of PCR?

Answer 15

To amplify DNA, creating millions of copies from a small sample.

Question 16

How does gel electrophoresis separate DNA fragments?

Answer 16

By applying an electric current, with smaller fragments moving faster through the gel toward the positive electrode.

Question 17

Why is a DNA ladder used in gel electrophoresis?

Answer 17

A DNA ladder contains fragments of known sizes, helping to estimate the size of the DNA bands.

Question 18

What is the role of primers in PCR?

Answer 18

Primers are short DNA sequences that bind to the template, marking the starting point for replication.

Question 19

What is the optimal temperature for the extension step?

Answer 19

72°C.

Question 20

List three applications of PCR and gel electrophoresis.

Answer 20

1. Forensic science
2. Medical diagnostics
3. Genetic research.