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Prepared By: Vipin Kumar Shukla
Assistant Lecturer.
POLYMERASE CHAIN REACTION(PCR)
What is PCR:?
ď‚— PCR is a technique that takes specific sequence of
DNA of small amount and amplifies it to be used for
further testing.
ď‚— In vitro technique
ď‚— As is the photo copier a basic requirement in an office,
so is the PCR machine in a molecular biology
Laboratory !!!!!!!!!
 PCR is DNA replication in a test tube……..
Short History of PCR:
ď‚— 1983: Dr. Kary Mullis developed PCR
ď‚— 1985: First publication of PCR by Cetus Corporation
appears in Science.
ď‚— 1986: Purified Taq polymerase is first used in PCR
ď‚— 1988: PerkinElmer introduces the automated thermal
cycler.
ď‚— 1989: Science declares Taq polymerase "molecule of the
year.
Continued…….
ď‚— 1990: amplification and detection of specific DNA
sequences using a fluorescent DNA-binding dye, laying the
foundation for future "real-time" or "kinetic" PCR.
ď‚— 1991: RT-PCR is developed using a single thermo stable
polymerase, rTth, facilitating diagnostic tests for RNA
viruses.
ď‚— 1993:Dr. Kary Mullis shares Nobel Prize in Chemistry for
conceiving PCR technology.
Continued…..
ď‚— 1999: Dynal launches DRB-36 HLA-typing kit for tissue
typing.
ď‚— 2003: HIV-1 MONITOR Test, version 1.5 Product Family
 AMPLICOR® CT/NG Test for Chlamydia trachomatis,
 AMPLICOR® CT/NG Test for Neisseria gonorrhea
Principle of PCR:
ď‚— Purpose:
ď‚— Condition:
ď‚— Components:
Purpose of PCR:
ď‚— To amplify a lot of double-stranded DNA
molecules (fragments) with same (identical) size
and sequence by enzymatic method and cycling
condition.
Condition:
ď‚— 1. Denaturation of double stranded DNA
template
ď‚— 2. Annealing of primers
ď‚— 3. Extension of double stranded DNA molecules
Basic requirements for PCR
reaction :
ď‚— 1) DNA sequence of target region must be known.
ď‚— 2) Primers - typically 20-30 bases in size. These can be
readily produced by commercial companies. Can also be
prepared using a DNA synthesizer
ď‚— 3) Thermo-stable DNA polymerase - e.g. Taq polymerase
which is not inactivated by heating to 95 °C
ď‚— 4) DNA thermal cycler - Machine which can be
programmed to carry out heating and cooling of samples
over a number of cycles.
Instrumentation:
Three Aspects of PCR:
ď‚— Specificity:
ď‚— Efficiency:
ď‚— Fidelity:
Tricks to follow if PCR not works:
ď‚— A)If no product ( of correct size ) produced:
ď‚— 1 Check DNA quality
ď‚— 2 Reduce annealing temperature
ď‚— 3 Increase magnesium concentration
ď‚— 4 Add dimethylsulphoxide ( DMSO ) to assay ( at around
10% )
ď‚— 5 Use different thermostable enzyme
ď‚— 6 Throw out primers - make new stocks
Continued……
ď‚— B) If extra spurious product bands present
ď‚— 1 Increase annealing temperature
ď‚— 2 Reduce magnesium concentration
ď‚— 3 Reduce number of cycles
ď‚— 4 Try different enzyme
Example of PCR program me:
 Initial Denaturation 95°C for 5 mins
ď‚— Thermo-cycle file 30 cycles of
 Denaturation : 95°C for 30 secs
 Annealing : 55°C for 30 secs
 Extension : 72°C for 45 secs
 Final extension 72°C for 5 mins
 Holding ( soak ) file usually 4°C
Advantages of PCR:
ď‚— Small amount of DNA is required per test
ď‚— Result obtained more quickly - usually within 1 day for PCR
ď‚— Usually not necessary to use radioactive material (32P) for PCR.
ď‚— PCR is much more precise in determining the sizes of alleles -
essential for some disorders.
ď‚— PCR can be used to detect point mutations.
Applications of PCR:
Continued…..
Polymerase chain reaction(pcr)

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Polymerase chain reaction(pcr)

  • 1. Prepared By: Vipin Kumar Shukla Assistant Lecturer. POLYMERASE CHAIN REACTION(PCR)
  • 2. What is PCR:? ď‚— PCR is a technique that takes specific sequence of DNA of small amount and amplifies it to be used for further testing. ď‚— In vitro technique ď‚— As is the photo copier a basic requirement in an office, so is the PCR machine in a molecular biology Laboratory !!!!!!!!! ď‚— PCR is DNA replication in a test tube……..
  • 3. Short History of PCR: ď‚— 1983: Dr. Kary Mullis developed PCR ď‚— 1985: First publication of PCR by Cetus Corporation appears in Science. ď‚— 1986: Purified Taq polymerase is first used in PCR ď‚— 1988: PerkinElmer introduces the automated thermal cycler. ď‚— 1989: Science declares Taq polymerase "molecule of the year.
  • 4. Continued……. ď‚— 1990: amplification and detection of specific DNA sequences using a fluorescent DNA-binding dye, laying the foundation for future "real-time" or "kinetic" PCR. ď‚— 1991: RT-PCR is developed using a single thermo stable polymerase, rTth, facilitating diagnostic tests for RNA viruses. ď‚— 1993:Dr. Kary Mullis shares Nobel Prize in Chemistry for conceiving PCR technology.
  • 5. Continued….. ď‚— 1999: Dynal launches DRB-36 HLA-typing kit for tissue typing. ď‚— 2003: HIV-1 MONITOR Test, version 1.5 Product Family ď‚— AMPLICOR® CT/NG Test for Chlamydia trachomatis, ď‚— AMPLICOR® CT/NG Test for Neisseria gonorrhea
  • 6. Principle of PCR: ď‚— Purpose: ď‚— Condition: ď‚— Components:
  • 7. Purpose of PCR: ď‚— To amplify a lot of double-stranded DNA molecules (fragments) with same (identical) size and sequence by enzymatic method and cycling condition.
  • 8. Condition: ď‚— 1. Denaturation of double stranded DNA template ď‚— 2. Annealing of primers ď‚— 3. Extension of double stranded DNA molecules
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  • 16. Basic requirements for PCR reaction : ď‚— 1) DNA sequence of target region must be known. ď‚— 2) Primers - typically 20-30 bases in size. These can be readily produced by commercial companies. Can also be prepared using a DNA synthesizer ď‚— 3) Thermo-stable DNA polymerase - e.g. Taq polymerase which is not inactivated by heating to 95 °C ď‚— 4) DNA thermal cycler - Machine which can be programmed to carry out heating and cooling of samples over a number of cycles.
  • 18. Three Aspects of PCR: ď‚— Specificity: ď‚— Efficiency: ď‚— Fidelity:
  • 19. Tricks to follow if PCR not works: ď‚— A)If no product ( of correct size ) produced: ď‚— 1 Check DNA quality ď‚— 2 Reduce annealing temperature ď‚— 3 Increase magnesium concentration ď‚— 4 Add dimethylsulphoxide ( DMSO ) to assay ( at around 10% ) ď‚— 5 Use different thermostable enzyme ď‚— 6 Throw out primers - make new stocks
  • 20. Continued…… ď‚— B) If extra spurious product bands present ď‚— 1 Increase annealing temperature ď‚— 2 Reduce magnesium concentration ď‚— 3 Reduce number of cycles ď‚— 4 Try different enzyme
  • 21. Example of PCR program me: ď‚— Initial Denaturation 95°C for 5 mins ď‚— Thermo-cycle file 30 cycles of ď‚— Denaturation : 95°C for 30 secs ď‚— Annealing : 55°C for 30 secs ď‚— Extension : 72°C for 45 secs ď‚— Final extension 72°C for 5 mins ď‚— Holding ( soak ) file usually 4°C
  • 22. Advantages of PCR: ď‚— Small amount of DNA is required per test ď‚— Result obtained more quickly - usually within 1 day for PCR ď‚— Usually not necessary to use radioactive material (32P) for PCR. ď‚— PCR is much more precise in determining the sizes of alleles - essential for some disorders. ď‚— PCR can be used to detect point mutations.