DNA Profiling Flashcards

1
Q

How is a DNA profile created? [basic explanation - 4]

A
  • DNA sample obtained
  • PCR amplifies specific regions of DNA
  • Fluorescent tag added to all DNA fragments so can be viewed under UV light
  • Gel electrophorisis seperates DNA fragments according to length
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2
Q

How can a DNA profile be analysed?

A
  • DNA fragments appear as bands under UV light making up a DNA profile
  • Two DNA profiles can be compared to see how similar the pattern of bands on the gel is
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3
Q

What do the bands on a DNA profile being in the same position mean?

A

The two chromosomes have the same number of STRs at a locus

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4
Q

What do the bands on a DNA profile being in different positions?

A

The two chromosomes have a different number of STRs at a locus

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5
Q

What are the 6 possible uses of DNA profiling?

A
  • Forensics
  • Evolutionary relationships between organisms
  • To prevent interbreeding in animals and plants
  • ID purposes
  • Paternity dispute
  • Forensics
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6
Q

How can DNA profile be used in forensics? 2

A
  • Compare DNA sample from crime scene to DNA samples from possible suspects
  • If samples match links person to crime scene
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7
Q

How can DNA profiling be used in paternity disputes? (3)

A
  • 1/2 of DNA comes from each parent
  • STRs are inherited like alleles - offspring receives 1 repeated sequence randomly from each parent
  • More bands on 2 DNA profiles matching - the more closely related the 2 people are
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8
Q

Why should interbreeding in plants and animals be prevented? 2

A
  • Decreases gene pool so increased risk of genetic disorders
  • Could cause health, productivity and reproductive problems
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9
Q

What is the flaw in DNA profiling?

A

DNA profile only analyses a few repeated sequences out of genome - less likely to be unique to each person

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10
Q

What is the purpose of PCR? 2

A
  • To amplify DNA for there to be enough to make a DNA profile
  • By making millions of copies of specific regions of DNA
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11
Q

What does the PCR reaction mixture contain? 4

A
  • DNA primers
  • Free DNA nucleotides
  • DNA polymerase
  • DNA sample
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12
Q

What are primers?

A

Short DNA sequences complementary to bases adjacent to STR

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13
Q

Why are primers needed in PCR?

A

To provide an OH group as the starting point for DNA polymerase to attach bases in creating a new DNA strand

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14
Q

Why are 2 different primers needed in PCR? 2

A
  • Each primer binds to one end of the DNA segment to be amplified
  • The sequence at the two ends is different
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15
Q

Explain the steps of PCR - 8

A
  • Reaction mixture is heated to 95c, breaking the hydrogen bonds between the two DNA strands so they separate into 2
  • Mixture is cooled to 55c to allow primers to anneal [bind to] to strands at the start of the STR with complementary base pairing
  • Heated to 70c – the optimum temperature for DNA polymerase
  • DNA polymerase lines up free nucleotides alongside the DNA template strand so new complementary strands are formed
  • Two copies of the DNA fragment formed as 1 cycle of PCR is complete
  • Cycle starts again as mixture is heated to 95c and so all 4 DNA fragments are used as templates
  • Procedure repeated multiple times
  • Each PCR doubles amount of DNA
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16
Q

What is the purpose of gel electrophoresis?

A

Used to separate out DNA fragments according to length

17
Q

Explain gel electrophoresis - 6

A
  • DNA placed in a well that is cut into an agrose gel
  • Covered in buffer solution conducting electricity
  • Gel connected to electrodes
  • Electrical current applied
  • DNA fragments positively charged so move to anode at far end of the gel
  • Short DNA fragments move faster and further towards anode
18
Q

What is the size of a DNA fragment determined by?

A

Number of base pairs