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PCR Polymerase Chain Reaction

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PCR

Polymerase Chain Reaction

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Invented by Kary Mullis

Mullis and Faloona, 1987. Specific synthesis of DNA in vitro via a

polymerase-catalyzed chain reaction.

Nobel Prize 1993

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Kary Mullis himself….

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“I was working for Cetus, making oligonucleotides. They were heady times. Biotechnology was in flower and one spring night while the California buckeyes were also in flower I came across the polymerase chain reaction. I was driving with Jennifer Barnett to a cabin I had been building in northern California. She and I had worked and lived together for two years. She was an inspiration to me during that time as only a woman with brains, in the bloom of her womanhood, can be. That morning she had no idea what had just happened. I had an inkling. It was the first day of the rest of my life.”- from Karry Mullis’s autobiography at the Nobel e-Museum

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PCR

Specifically targets and amplifies a SINGLE sequence from within a complex

mixture of DNA.

How is this different from cloning?

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Takes advantage of basic requirements of replication

A DNA template NucleotidesPrimerspolymerase

PCR is DNA replication in a test tube

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PrimersMust have some information about sequence flanking your target

Primers provide specificity

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5’

5’

3’

3’

Complementary to opposite strands with 3’ ends pointing towards each other

Should have similar melting temperatures

Be in vast excess

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Melting temperature

TmoC = 2(A/T) + 4(G/C)

TmoC Temperature at which

half possible H bonds are formed

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The basic process

dsDNA

Denature (95 degrees)

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5’

5’

3’

3’

http://www.dnalc.org/shockwave/pcranwhole.html

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Thermocycling

94 degrees55 degrees70 degree

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Heat-stable polymerase is vital to the ease of the process…

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Thermus aquaticus:

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The Thermus aquaticus DNA polymerase

Taq

Not permanently destroyed at 94ºCOptimal temperature is 72ºC

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Problems with Taq

Does not have proof readng ability Error rate 1 in 2 X 104 basesSeems rare but can be recovered in cloning a single moleculeNewer polymerases have high fidelity

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Termplates for PCR

Small amount of templateIn theory a single moleculeDo not need to isolate sequence of interestDNA template need not be highly purifiedDNA is stable in absence of nucleases

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Templates for PCR

Dried bloodSemen stains

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Templates for PCRDried bloodSemen stainsVaginal swabsSingle hairFingernail scrapingsInsects in AmberEgyptian mummiesBuccal SwabToothbrushes

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PCR variations

Add 5’ extensions for cloning5’ 3’

5’3’

TC

A

3’

3’

5’

AA

T

G

TC

5’

TA

G

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Cloning PCR Fragments

Taq leaves 3’ A overhang.

AA

TT

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rtPCR

Reverse trancriptase PCR

Use mRNA as a template

Isolated cDNA clones

Can be quantitative

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Inverse PCR

known unknown

Knownunknown unknown

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known

unknown

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Nested primers

PCR primers are not always an exact match!

Degeneracy

Lower annealing temperatures increase chances of amplifying something!

Could be wrong thing!

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Nested primers

1

12

2

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Quantitative PCR

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Real Time PCR

Detection and quantitation of fluorescent reporter the signal of which increases in direct proportion to the

amount of PCR product in a reaction

Does not measure the amount of end product but its production in real time

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SYBRgreen

Also binds primer dimersCan overestimate product

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Molecular Beacons

Uses FRETFuorescence Resonance Energy TransferUses two sequence specificoligonucleotides labeled with fluorescent dyes

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Taq Man

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Other application of PCR

Detection of mutationsscreen for inherited disorders

Detection of HIVNot standard test given

Detect tuberculosis without culturingPrenatal sex determination

DZY1 = Y specific sequence present in 5000 copies

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Other application of PCR

Preimplantation diagnosis of genetic diseasesForensicsPaternity testing

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ForensicsSTRShort Tandem Repeats

2 to 7 base pairs repeated 7-40 timesReplaced VNTRs in forensic analysis

13 Highly polymorphic loci have been selected by FBI

Population match probabilities 0.1 - 0.28Probability One in 5.7 X 10-15

Combined DNA Index System (CODIS)

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STR analysis of family of last Tsar of Russia

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VNTR’s

Can use PCR to visualize VNTRs

Eg. pMCT118 in chromosome 1

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VNTR analysis

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Problems with PCR

ContaminationTheoretically one molecule can amplifyTakes one mismatch early on to amplify the wrong fragment