Presentation is loading. Please wait.

Presentation is loading. Please wait.

Random Amplified Polymorphic DNA RAPD

Published byPiers Singleton Modified over 6 years ago

Similar presentations

Presentation on theme: "Random Amplified Polymorphic DNA RAPD"— Presentation transcript:

1 Random Amplified Polymorphic DNA RAPD

2 History Shortly after Kary Mullis invented the Polymerase Chain Reaction (PCR) it was realized that short primers would bind to several locations in a genome and thus could produce multiple fragments Williams et al. (1990) developed Random Amplified Polymorphic DNA (RAPD) a technique using very short 10 base primers to generate random fragments from template DNAs RAPD fragments can be separated and used as genetic markers or a kind of DNA fingerprint Techniques related to RAPD include: DNA Amplification Fingerprinting (DAF) - Caetano-Anolles et al. (1991) uses very short (eight nucleotide long) primers Arbitrary Primed PCR (AP-PCR) - Welsh and McClelland (1990) uses longer primers, but lowers primer annealing stringency to get priming at many sites

3 Components of a PCR and RAPD Reactions
Buffer (containing Mg++) - usually high Mg++ concentrations are used lowering annealing stringency Template DNA 1 short primer (10 bases) not known to anneal to any specific part of the template DNA dNTPs Taq DNA Polymerase (or another thermally stable DNA polymerase) PCR Buffer (containing Mg++) Template DNA 2 Primers that flank the fragment of DNA to be amplified dNTPs Taq DNA Polymerase (or another thermally stable DNA polymerase)

4 DNA Between The Primers Doubles With Each Thermal Cycle
Cycles Number 1 1 2 2 4 3 8 4 16 5 32 6 64

5 Modifying Thermal Cycling
Two modifications made to typical thermal cycling when RAPD is being done: Annealing temperatures are generally very low, around 36 oC - This allows very short primers to anneal to template DNA More thermal cycles are used, typically 45 - This compensates for the inefficiency which results from using such short primers.

6 RAPD Primer binds to many locations on the template DNA
Only when primer binding sites are close and oriented in opposite direction so the primers point toward each other will amplification take place

7 RAPD Primers point away from each other, so amplification won’t happen
Template DNA Primers point away from each other, so amplification won’t happen

8 RAPD Template DNA Primers point in the same direction, so amplification won’t happen

9 RAPD Template DNA > 2,000 bases Primers too far apart, so amplification won’t happen

10 RAPD Template DNA Primers are just the right distance apart, so fragment is amplified ,500 bases

11 Separated RAPD Fragments
4mM MgCl2 1.2 U Taq 5 pM OPA-16 4mM MgCl2 0.6 U Taq 10 pM OPA-16 2mM MgCl2 1.2 U Taq 10 pM OPA-16 RAPD reactions were run in groups of 3 using the same template and primer, but varying Magnesium, polymerase and primer concentrations Which variable has the greatest impact on fragment patterns? M Lowering Magnesium ion concentration results in loss of the largest fragment visible in lanes 2-7 Normal concentrations are shown in yellow text. M = A size standard

Download ppt "Random Amplified Polymorphic DNA RAPD"

Similar presentations

RAPD Randomly Amplified Polymorphic DNA

RAPD Randomly Amplified Polymorphic DNA
Polymerase Chain Reaction (PCR)

Polymerase Chain Reaction (PCR)
Polymerase Chain Reaction (PCR). PCR produces billions of copies of a specific piece of DNA from trace amounts of starting material. (i.e. blood, skin.

Polymerase Chain Reaction (PCR). PCR produces billions of copies of a specific piece of DNA from trace amounts of starting material. (i.e. blood, skin.
DNA Fingerprinting and Forensic Analysis Chapter 8.

DNA Fingerprinting and Forensic Analysis Chapter 8.
PCR Basics Purpose of PCR Overview Components of PCR Reaction

PCR Basics Purpose of PCR Overview Components of PCR Reaction
PCR Basics 1.Purpose of PCR 2.Overview 3.Components of PCR Reaction 4.Variables Temperature Cycle Times and Numbers Primer Buffer Polymerase 5.Experimental.

PCR Basics 1.Purpose of PCR 2.Overview 3.Components of PCR Reaction 4.Variables Temperature Cycle Times and Numbers Primer Buffer Polymerase 5.Experimental.
PCR Polymerase Chain Reaction. PCR - a method for amplifying (copying) small amount of DNA in nearly any amount required, starting with a small initial.

PCR Polymerase Chain Reaction. PCR - a method for amplifying (copying) small amount of DNA in nearly any amount required, starting with a small initial.
PCR. PCR AMPLIFICATION PCR APPLICATIONS b MOLECULAR BIOLOGY b ENVIRONMENTAL SCIENCE b FORENSIC/MEDICAL SCIENCE b BIOTECHNOLOGY b GENETICS b GENE CLONING.

PCR. PCR AMPLIFICATION PCR APPLICATIONS b MOLECULAR BIOLOGY b ENVIRONMENTAL SCIENCE b FORENSIC/MEDICAL SCIENCE b BIOTECHNOLOGY b GENETICS b GENE CLONING.
PCR Overview Lifted from various powerpoint presentations on the internet.

PCR Overview Lifted from various powerpoint presentations on the internet.
General Genetics. PCR 1.Introduce the students to the preparation of the PCR reaction. PCR 2.Examine the PCR products on agarose gel electrophoresis.

General Genetics. PCR 1.Introduce the students to the preparation of the PCR reaction. PCR 2.Examine the PCR products on agarose gel electrophoresis.
The PCR The Polymerase Chain Reaction. The PCR is used to make copies of DNA (amplification). Whole genome OR DNA fragments.

The PCR The Polymerase Chain Reaction. The PCR is used to make copies of DNA (amplification). Whole genome OR DNA fragments.
The polymerase chain reaction (PCR) rapidly

The polymerase chain reaction (PCR) rapidly
ZmqqRPISg0g&feature=player_detail page The polymerase chain reaction (PCR)

ZmqqRPISg0g&feature=player_detail page The polymerase chain reaction (PCR)
Accuracy: The closeness of a measured volume to the true volume as specified by the volume setting of the pipette. Also known as “mean error”. precision:

Accuracy: The closeness of a measured volume to the true volume as specified by the volume setting of the pipette. Also known as “mean error”. precision:
Polymerase Chain Reaction

Polymerase Chain Reaction
Polymerase Chain Reaction (PCR) is when you amplify the number of copies of a specific region of DNA, in order to produce enough DNA it be adequately.

Polymerase Chain Reaction (PCR) is when you amplify the number of copies of a specific region of DNA, in order to produce enough DNA it be adequately.
WORKSHOP (1) Presented by: Afsaneh Bazgir Polymerase Chain Reaction

WORKSHOP (1) Presented by: Afsaneh Bazgir Polymerase Chain Reaction
Advanced Molecular Biological Techniques. Polymerase Chain Reaction animation.

Advanced Molecular Biological Techniques. Polymerase Chain Reaction animation.
©2001 Timothy G. Standish Romans 5:17 17For if by one man’s offence death reigned by one; much more they which receive abundance of grace and of the gift.

©2001 Timothy G. Standish Romans 5:17 17For if by one man’s offence death reigned by one; much more they which receive abundance of grace and of the gift.
Recombinant DNA Technology………..

Recombinant DNA Technology………..

Similar presentations

Ads by Google