03 - Lecture 18

Question 1

What help you see the changes in DNA?

Answer 1

Probes, fluorence

Question 2

What happens if there is a mutation in the promoter region?

Answer 2

The RNA polymerase will not see the promoter region and will not make RNA to begin with

Question 3

Gel electrophoresis?

Answer 3

Top is big and bottom is small

Question 4

What is used to chop up the DNA into fragments?

Answer 4

Restriction endonuclease

Question 5

Does Northern blot use a restriction endonuclease?

Answer 5

No because RNA is single stranded

Question 6

What helps isolate mRNA from the cell?

Answer 6

Poly-T tail attached to a bead

Question 7

What is the charge of the proteins when doing Western blot?

Answer 7

The proteins are negatively charged because of the detergent that coats the proteins

Question 8

What technique would you use if you do not know what the mutation is?

Answer 8

di-deoxy method

Question 9

Base pairs are incorporated in to a growing chain until what?

Answer 9

Synthesis stops because of ddNTP (no 3’ OH)

Question 10

Steps of PCR?

Answer 10

Denature with heat into single strand DNA, the primer anneals to complementary DNA with cool temp, then you elongate the sample with warm temp

Question 11

Steps of RFLP?

Answer 11

Use a restriction endonuclease to recognize and cut a certain base sequence in the DNA (different genes = different length of fragments)
- after you cut out the fragments you can use Southern blotting to compare sizes

Question 12

How can southern blotting/RFLP be used for sickle cell?

Answer 12

In a normal beta globin gene there are two fragments (1.15 and 0.2) in the sickle cell fragment there is only one fragment (1.35)