DNA profiling Flashcards

Question 1

Q

STEP 1 - How would you extract the DNA?

Answer

A

The DNA is extracted from cells, tissues, blood
The DNA is purified
tiny amounts are needed because the lab techniques can copy the DNA as many times

Question 2

Q

Why does the DNA need to be purified?

Answer

A

Question 3

Q

STEP 2 - How would you digest the same with enzymes?

Answer

A

DNA sample is cut into smaller fragments using RESTRICTION ENZYME
They cut both stands and specific enzymes can be chose to cut the DNA at the start of a particular VNTR’s or STR’s that we are looking for.
This results in different lengths of fragments

Question 4

Q

STEP 3 - How would you separate the DNA fragments?

Answer

A

GEL ELECTROPHORESIS
DNA fragments are put into a well block of gel, along with loading dye to make them visible
placed into alkaline buffer solution which regulated PH and helps carry electrical charge across the gel
DNA fragments move towards the positive end (the phosphate groups in the DNA give it a negative charge)
smaller fragments move the furthest

Question 5

Q

Why do the fragments need to be separated?

Answer

A

Question 6

Q

Why is loading gel needed?

Answer

A

Question 7

Q

STEP 4 - What is hybdrisation?

Answer

A

DNA probes are added to look for a particular mini/micro - satellites in the DNA
the probes have complementary base sequence to look for the sequence you are looking for.
They are 100 - 1000 nucleotides long

Question 8

Q

How would you see the evidence/ make it visible?

Answer

A

If the probes are used a radioactive or fluorescent then they can be detected wherever they have attached
Radioactive probes - placing nylon membranes on a x-ray film causes the film to fog
fluorecent - place the nylon membrane under the uv light and the probes will glow

Question 9

Q

What happens if you place the probes on a fluorescent dye?

Answer

A

Question 10

Q

What happens if you place the probes on a x -ray film?

Answer

A

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