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Biology Y2 > 3.8.4 Gene technologies > Flashcards

3.8.4 Gene technologies Flashcards

1
Q

What is recombinant DNA technology?

A
  • transfer of fragments of DNA from one organism to another
  • possible because genetic code is universal
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2
Q

Describe the reverse transcriptase method for isolating DNA fragments

A
  • start with mRNA
  • use reverse transciptase enzyme to create cDNA (complementary DNA), which is single stranded
  • use DNA polymerase to create double stranded DNA
  • ends in a gene with no introns, no sticky ends
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3
Q

Describe the restriction endonuclease method for isolating DNA fragments

A
  • starts with DNA
  • cut out the gene using restriction endonucleases
  • restriction endonucleases are enzymes that cut at specific recognition sites
  • which are palindromes
  • to leave blunt or sticky ends
  • results in gene WITH introns
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4
Q

Describe the gene machine method for isolating DNA fragments

A
  • starts with polypeptide
  • use gene machine to synthesise required DNA sequence
  • can add promoter and terminator regions and restriction endonucleases sites on either side of DNA base sequence
  • no enzymes required
  • no introns, yes sticky ends
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5
Q

What does PCR stand for?

A

Polymerase chain reaction

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6
Q

What 4 things are added to the test tube before it enters the thermocycler (pcr) machine?

A
  • DNA fragment to be copied
  • DNA polymerase - to join adjacent DNA nucleotides in a phosphodiester bond to make complementary DNA strand
  • primers - to anneal the DNA fragments and provide a starting attachment point for DNA polymerase
  • DNA nucleotides - monomers to make the complementary strand of DNA to the original DNA fragment
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7
Q

Describe the PCR process

A
  • DNA heated to 95C
  • to break the hydrogen bonds between complementary DNA base nucleotides by heat, so the stands separate
  • cooled to 55C
  • annealing (binding) of primers
  • to provide a starting point for DNA polymerase to extend from
  • nucleotides attached
  • by complementary base pairing
  • 72C
  • optimum temperature for DNA polymerase
  • DNA polymerase joins adjacent nucleotides together with phosphodiester bonds
  • cycle repeats
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8
Q

Compare the similarities of a probe and a primer

A
  • both short
  • single stranded DNA sequences
  • complementary to DNA target sequence of interest
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9
Q

What are the differences between a probe and a primer

A
  • probe has a fluorescent or radioactive label, primer has no label
  • probe used to identify presence of DNA fragment/gene, primer used to start DNA synthesis by acting as a binding site for DNA polymerase
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10
Q

What are the facts genetic fingerprinting relies on?

A
  • each individuals DNA is unique
  • 95% of DNA is introns and non-coding sections between genes
  • non coding DNA have hypervariable regions that contain repetitive sequences- VNTR sequences (mini/microsatellites)
  • these vary in length and have a unique pattern
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11
Q

Genetic fingerprinting process

A
  • DNA extracted from sample, PCR amplifies DNA quantity
  • DNA cut into sections using restriction endonucleases
  • must leave required core VNTR sequences intact
  • DNA fragments separated by gel electrophoresis according to length
  • 2 strands of DNA separated by immersing gel in alkaline solution (dsDNA to ssDNA)
  • southern blotting- transfer gel to nylon membrane, DNA fixed to nylon membrane with UV light
  • radioactive probe added - only binds to complementary core VNTR sequences
  • X Ray film/autoradiography to identify areas the probe has bound
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12
Q

Uses of genetic fingerprinting

A
  • forensic science
  • paternity test
  • determine genetic variability in a population
  • medical diagnosis
  • plant and animal breeding
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13
Q

Gel electrophoresis process

A
  • DNA negatively charged, moves towards positive electrode
  • longer fragments move more slowly through gel, shorter fragments move more quickly
  • distance moved depends on length/number of base pairs
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14
Q

In vivo cloning: use of vectors

A
  • restriction endonucleases cut at recognition sites leaving sticky ends
  • DNA fragment modified to ensure transcription- promoter and terminator regions added
  • insert DNA into a vector- plasmids:
  • plasmid cut with same restriction endonuclease to create same sticky ends
  • DNA fragment and plasmid combined with enzyme ligase (anneals them)
  • plasmid with recombinant DNA inserted into host cell:
  • Heat shock host cells to increase permeability of host cell membrane
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15
Q

Using a radioactove probe

A
  • extract DNA and add restriction endonucleases
  • separate fragments using electrophoresis
  • treat DNA to form single strands
  • the probe will bind to the gene
  • use autoradiography to show the bound probe
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Biology Y2 (21 decks)

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