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gene technology > L2 PCR > Flashcards

L2 PCR Flashcards

1
Q

replisome

A

proteincomplex that handles replication in bacteria

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2
Q

DNA gyrase

A

releases tension in DNA to prevent twists and knots on DNA strands

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3
Q

DNA helicase

A

breaks apart dsDNA

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4
Q

DNA polymerase iii

A

performs replication on leading strand
downstream

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5
Q

DNA polymerase i

A

performs replication on lagging strand
upstream

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6
Q

dNTP
ddNTP

A
  • dNTP = dioxy NTP = sugar based, they have one extra OH-group

-ddNTP= they have no extra OH-group

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7
Q

nucelase, exonuclease

A
  • nuclease = breaks down nts
  • exonuclease = degrades nts, for ex. after there’s been a mistake
    -> DNAP has exonuclease acitivity
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8
Q

DNA ligase

A

connects fragments

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9
Q

PCR

A

= used to amplify DNA

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10
Q

primer

A

= synthesized DNA
- around 20 nts
-> too long: will form hairpins
-> too short: not specific enough, can bind anywhere and not just where you want it to

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11
Q

PCR general process

A

heat up DNA => dsDNA seperates
cool down DNA and hope primer anneals before complementary sequence

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12
Q

how does primer win “competition”?

A
  • 2 things competing:
    1. primer annealing to template strand
    2. complementary sequence annealing to template strand
  • primer wins because there’s a looot of primer which makes it favourable
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13
Q

adding overhangs

A

= a way to use PCR to add a sequence to another sequence

1st cycle: overhang (~20 nts) added to 5’-end of primer, primer anneals to template strand and gets replicated

2nd cycle: overhang has been added to DNA and new overhang can be added with new primer etc

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14
Q

overlap extension PCR

A

= used to add sequence to middle of target

step 1: add 4 primers, 2 to each strand, the two in the middle have complementary overhangs
=> 2 PCR reactions happen at once

step 2: the leading strand on one of the two dsDNA formed align with the lagging strand of the other (where DNAP can go 5’->3’) and DNAP performs replication so a new dsDNA is formed with the overhangs in the middle
-> the other strands can’t form new dsDNA since DNAP can’t go 3’->5’

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15
Q

problem with PCR (mutations)

A
  • Taq polymerase used => good! can handle 90 degrees Celcius
    -> but, has no proofreading
  • in lab: 15-20 cycles of PCR performed => many mutations which we can’t get rid of
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16
Q

solution to problem with PCR

A

= filtrate DNA!
- put all DNA into plasmids via ligation reaction
- transform plasmids into E. coli that takes up one plasmid each where it gets replicated
- some E. coli will then hold plasmids with no mutations
=> find them via DNA sequencing

gene technology (7 decks)

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