PCR workshop (Suitable for Edvotek kits 330, 371, 372) Edvotek Europe.

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PCR workshop (Suitable for Edvotek kits 330, 371, 372) Edvotek Europe

Transcript of PCR workshop (Suitable for Edvotek kits 330, 371, 372) Edvotek Europe.

Page 1: PCR workshop (Suitable for Edvotek kits 330, 371, 372) Edvotek Europe.

PCR workshop(Suitable for Edvotek kits 330, 371, 372)

Edvotek Europe

Page 2: PCR workshop (Suitable for Edvotek kits 330, 371, 372) Edvotek Europe.

What are we doing today?

• Introduction• Set up PCR reaction• Load gels• Electrophoresis• Analyse results

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Health & safety

• No toxic chemicals• Safe solutions and reagents used

in place of research materials

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The Polymerase Chain Reaction

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What does PCR do?

• PCR makes millions of copies of DNA

• Uses PCR machine• A DNA photocopier!

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Cell division

DNA polymerase duplicates DNA during cell division

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DNA polymerase in action!

Stars show DNA polymerase bound to DNA

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Who invented PCR?

Kary Mullis - inventor of PCR, Nobel Prize 1993

“EUREKA!!! I stopped the car. Somehow, I thought, it had to be an illusion.

Otherwise it would change DNA chemistry forever. Otherwise it would make me famous. It was too easy. Someone else would have done it and surely I would have heard of it.

We would be doing it all the time.”

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Mullis’s Nobel prize speech is well worth

readinghttp://www.nobelprize.org/

nobel_prizes/chemistry/laureates/1993/mullis-lecture.html

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What is in a PCR reaction

Use 5μl from tube labelled “Template DNA”

Use 20μl from tube labelled “primers”

The PCR bead

Template DNA The starting material in a PCR reaction.

Primers are two short pieces of DNA (0-15 bases long) that determine the region of DNA to be copied.

NucleotidesA’s, T’s, G’s and C’s to make up the new DNA strands

Taq DNA polymeraseThe enzyme that makes new DNA strands

MgCl2Required for Taq DNA polymerase to function

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Mix the following:

•Template DNA•Nucleotides•Primers•Taq DNA polymerase

•MgCl2

How does PCR work?

++ ++ ++

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Cycle through 3 temperatures

• Denature: unzips DNA

• Anneal: primers bind to complementary areas of target DNA

• Extend: Taq DNA polymerase fills in the blanks!

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Lots of DNA produced

• Successive cycles double amount of DNA

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Taq DNA polymerase

• Thermus aquaticus bacteria that lives at high temperature

• DNA polymerase crucial to automate PCR

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Uses of PCR

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Forensics!

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Paternity testing

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Genetic testing

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Types of PCR kit

• DNA template provided (intro level)– Cat no 371 DNA fingerprinting– Cat no 372 Quick PCR

• DNA template must be extracted (more advanced)– Cat no 333 or 334 chromosome kit

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The experiment

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Quick PCR set up

• Carefully transfer PCR bead to 0.2ml tube & label

• Add 5ul template DNA• Add 20ul primer mix• Place in PCR machine

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Quick PCR cycles

• Initial denaturation 94°C for 180 seconds

• Then 20 cycles of:94°C for 30 seconds71°C for 15 seconds (annealing)71°C for 15 seconds (extension)

• Annealing & extension are same temperature

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EdvoCycler

• PCR machine• Easy to use• Select cat no• Programmable

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Choose programme

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Press to select

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Lid will heat up

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Then cycles start

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Then cycles startProgramme selected = Cat no of kit

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Then cycles start

Number of cycles to go

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Then cycles start

Number of cycles completed

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Then cycles start

Temperature for each step

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Then cycles start

Time in seconds for each step

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DNA electrophoresis

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Gel casting

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Running buffer

TAE buffer• 20ml 50x buffer to 1 litre with

water

• Distilled water ideal but tap ok• Can be reused a few times• Store unused for future use ok

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Agarose

0.8% Agarose• 3g in 375 ml dilute buffer• Melt in microwave/autoclave• Pour when hand hot

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Agarose

• Store gels for 1-2 weeks in fridge wrapped in cling film or plastic bag

• Keep any left over gels and remelt next time

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Remove comb & ends

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Fixed volume minipipette

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Adjustable micropipette

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Dry loading• You can load gel dry instead of through

buffer!• Otherwise load “wet” through buffer

Either way, remember• Do not puncture bottom of well• Change tips between each sample

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HexaGel and EVT 300 power supply

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Quick PCR kit gel LoadingAfter PCR reaction add 5l loading dye

Load 40 l of each sample into the wells

A

M

B

LG1

C

LG2

D E F

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Run gels

• Put on lid and attach to power supply

• Run for 30 minutes at 150 volts• Or 75 volts for 40-50 minutes • Check for bubbles at electrode• Run until tracking dye halfway

across gel

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After gel run stain the gel

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Stain PCR gel

• MetBlue card blue side down 5 mins

• Weigh with gel tray• Destain in warm water 10-15 mins• Leave overnight in fridge for best

result• Keep long term in bag in fridge

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Stain Gel

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Gel storage

• Can store gels in fridge before staining over weeknight or weekend

• Cannot store dye kits overnight before viewing as diffuse!

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Quick PCR result

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Thank you

• PCR experiments can be carried out easily

• Fun and relevant to wider world• Promote understanding