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ANUSHA SHAJI, B.Pharm, M.Pharm
Assistant Professor
Department of Pharmacology
Nirmala College of Pharmacy,
Muvattupuzha, Ernakulam, Kerala
POLYMERASE CHAIN
REACTION
2
3
4
INTRODUCTION-PCR
 In genetic engineering , the availability of sufficient
amount of DNA of interest is indispensable in order to
study its structure , function and manipulation.
 Until recently the micro-organisms are the chief source
to obtain multiple copies of DNA of interest.
 Now a new and novel cell free technique are available
to obtain millions of copies, known as polymerase chain
reaction (PCR technique)
5
 PCR, polymerase chain reaction, is an in-vitro technique
that allows amplification of a particular DNA sequence
and is able to generate innumerable copies of specific
DNA sequence.
 The technique is so precise and powerful, that even a
single gene sequence can be amplified into a detectable
amount within a short time.
 The technique was independently designed and
developed by Karymullis in 1980.
6
-
7
1- DNA TEMPLATE
 DNA containing region
(target) to be sequenced
or amplified
 Size of target DNA to be
amplified : up to 3 Kb
8
2- PRIMERS
• 1 sets of primers
• Generally 20-30
nucleotides long
• Synthetically produced
• complimentary to the 3’
ends of target DNA
• not complimentary to each
other
9
3-ENZYME
 Usually Taq Polymerase or anyone of the natural or
Recombinant thermostable polymerases
 Taq polymerase – obtained from Thermus
aquaticus
 This enzyme,Taq polymerase has an optimum
temperature 72ᵒC and the enzyme remains stable
at 950 C
10
Another reason for using thermostable DNA polymerase
is that :
 DNA synthesised at high temperature is relatively more
error free than the DNA synthesised at ordinary
temperature like 25ᵒ to 30ᵒC.
11
DEOXYNUCLEOTIDE TRIPHOSPHATES
 The four nucleosides containing triphosphate groups;
dNTPs
They are the building-blocks from which the DNA
polymerase synthesizes a new DNA strand.
12
BUFFER SOLUTION
 Providing a suitable chemical environment for
optimum activity and stability of the DNA polymerase
Tris HCl , KCl , MgCl2 , Taq buffer etc can be used.
13
DIVALENT CATIONS
 Magnesium or manganese ions
 Generally Mg2+ is used, but Mn2+ can be utilized for
PCR mediated DNA mutagenesis
As higher Mn2+ concentration increases the error rate
during DNA synthesis
14
 PCR, POLYMERASE CHAIN REACTION, is an in-vitro
technique that allows amplification of a particular DNA
sequence and is able to generate innumerable copies
of specific DNA sequence.
15
PRINCIPLE
A characteristic feature of DNA is that bringing it to a
certain high temperature known as melting temperature
(Tm)
↓
The double strands fall apart into single strands by
dissolution of the H-bonds
↓
When the temperature is lowered , the two strands again
anneal to restore the double helix structure (annealing
temperature)
↓
PCR technique utilizes this property of DNA for replication
16
THE PCR MACHINE
 The PCR machine is a thermal cycler in which the
temperature , time and number of cycles required
for amplification of the sample DNA can be preset
for automatic operation.
 Normal DNA polymerase is thermo labile → a
thermo stable DNA polymerase obtained from a
thermophilic organism is used.
 This avoids the addition of the enzyme in each
cyclic operation.
17
PCR INSTRUMENT
18
THE PCR CYCLE
Comprised of 3 steps:
• Denaturation of DNA at 950C
• Primer hybridization ( annealing) at 40-500C
• DNA synthesis ( Primer extension) at 720C
19
DENATURATION
The first step is the
denaturation of DNA
sample in a reaction
mixture to 95 °C .
At this thermal condition
DNA strand gets
separated.
The temperature is
maintained up to 5
minutes.
20
RENATURATION
The temperature is
lowered to 50 °C to allow
the 2 oligonucleotide
primers to anneal (bind) to
the complementary
sequence in the DNA
molecule.
The time duration of 30
seconds is maintained for
renaturation.
21
SYNTHESIS OF NEW DNA
The temperature is
raised to 72-75 °C .
At this elevated
temperature , Taq
polymerase shows
optimum activity and
initiates DNA synthesis
at 3 hydroxyl end of each
primer.
22
23
24
STANDARD THERMOCYCLE
25
TYPES OF PCR
 Several modifications of PCR have been developed for
specific applications
 Another reason for the modification is to overcome
problems or trouble shooters during amplification.
 Following are some of the improved version of PCR.
 Nested PCR
 Inverse PCR
 Hot start PCR
26
1. NESTED PCR
 Nested PCR is a variation of the polymerase chain
reaction , in that 2 pairs ( instead of 1 pair) of PCR primers
are used to amplify a fragment.
TECHNIQUE
Step 1 : primers binds to template DNA and PCR start.
Step 2 : PCR products from the first PCR reaction are
subjected to a second PCR run.
Step 3 : we can get multiple copies
27
28
2. HOT-START PCR
A technique that reduces non-specific amplification
during the initial set up stages of the PCR.
It may be performed manually by heating the reaction
components to the melting temperature (eg.95ᵒC) before
adding the polymerase.
 2 types
a. Mechanical hot start b. non-mechanical hot start
29
 MECHANICAL HOT START PCR
All components of PCR are added to the PCR vial
except for the DNA polymerase enzyme which will be
added just at the first denaturation step.
 NON-MECHANICAL HOT START PCR
The use of a form of Taq DNA polymerase , for
example , Amplitaq Gold which is activated only if the
reaction mixture is heated at about 94ᵒC ( the first
denaturation step)
30
 Other methods depend on covalent linking of the
polymerase enzyme to certain inhibitors.
The enzyme becomes dissociated from these
inhibitors at the first denaturation step.
31
32
HOT START PCR
33
3. INVERSE PCR
Target DNA is lightly cut into smaller fragments of
several kilobases by restriction endonuclease digestion.
Self-ligation is induced under low concentrations causing
the phosphate backbone to reform.
This gives a circular DNA ligation product.
Target DNA is then restriction digested with a known
endonuclease.
34
This generates a cut within the known internal
sequence generating a linear product with known
terminal sequences.
This can now be used for PCR (polymerase chain
reaction)
35
INVERSE PCR
36
OTHER VARIATIONS OF THE PCR
Colony PCR
Multiplex PCR
Asymmetric PCR
Long PCR
Allele specific PCR
Real time PCR
Reverse transcriptase PCR (RT-PCR)
In situ PCR
Long accurate PCR
Touch down PCR
AFLP PCR
37
• Automated, fast, reliable (reproducible) results
• High output
• Sensitive
• Broad uses
• Defined, easy to follow protocols
• Commercial kits are now available for easy PCR
reaction setup and amplification
ADVANTAGES
38
DISADVANTAGES
• Extreamly liable to contamination
• High degree of operator skills required
• False positive results due to amplifications
• Expensive to the developing world
39
APPLICATIONS
• It is extensively used for the amplification of a particular
target DNA sequence
• Genome mapping and gene function determination
• Biodiversity studies ( e.g. evolution studies)
• Detection of drug resistance genes
• In plant biotechnology, PCR is used in plant disease
identification , presence of any target gene in crop plants
40
• The PCR is widely employed in disease diagnosis (early
detection of cancer, viral infections...) .
• The speed and sensitivity of PCR helps in prenatal
diagnosis of inherited disease.
• Forensic (DNA fingerprinting)
• PCR has an important role in gene manipulation and
expression studies.
41
REFERENCE
 Biotechnology-4 by S. Mahesh and A.B Vedamurthy
, Page number : 32-35
 Ananthanarayanan and Paniker’s text book of
microbiology , 7th edition. C K J Paniker. Page
number : 591
 Molecular biology and biotechnology , 5th edition.
John M Walker and Ralph Rapley. Page number : 15-
18
 www.wikipedia.com
42

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Polymerase chain reaction

  • 1. 1 ANUSHA SHAJI, B.Pharm, M.Pharm Assistant Professor Department of Pharmacology Nirmala College of Pharmacy, Muvattupuzha, Ernakulam, Kerala POLYMERASE CHAIN REACTION
  • 2. 2
  • 3. 3
  • 4. 4 INTRODUCTION-PCR  In genetic engineering , the availability of sufficient amount of DNA of interest is indispensable in order to study its structure , function and manipulation.  Until recently the micro-organisms are the chief source to obtain multiple copies of DNA of interest.  Now a new and novel cell free technique are available to obtain millions of copies, known as polymerase chain reaction (PCR technique)
  • 5. 5  PCR, polymerase chain reaction, is an in-vitro technique that allows amplification of a particular DNA sequence and is able to generate innumerable copies of specific DNA sequence.  The technique is so precise and powerful, that even a single gene sequence can be amplified into a detectable amount within a short time.  The technique was independently designed and developed by Karymullis in 1980.
  • 6. 6 -
  • 7. 7 1- DNA TEMPLATE  DNA containing region (target) to be sequenced or amplified  Size of target DNA to be amplified : up to 3 Kb
  • 8. 8 2- PRIMERS • 1 sets of primers • Generally 20-30 nucleotides long • Synthetically produced • complimentary to the 3’ ends of target DNA • not complimentary to each other
  • 9. 9 3-ENZYME  Usually Taq Polymerase or anyone of the natural or Recombinant thermostable polymerases  Taq polymerase – obtained from Thermus aquaticus  This enzyme,Taq polymerase has an optimum temperature 72ᵒC and the enzyme remains stable at 950 C
  • 10. 10 Another reason for using thermostable DNA polymerase is that :  DNA synthesised at high temperature is relatively more error free than the DNA synthesised at ordinary temperature like 25ᵒ to 30ᵒC.
  • 11. 11 DEOXYNUCLEOTIDE TRIPHOSPHATES  The four nucleosides containing triphosphate groups; dNTPs They are the building-blocks from which the DNA polymerase synthesizes a new DNA strand.
  • 12. 12 BUFFER SOLUTION  Providing a suitable chemical environment for optimum activity and stability of the DNA polymerase Tris HCl , KCl , MgCl2 , Taq buffer etc can be used.
  • 13. 13 DIVALENT CATIONS  Magnesium or manganese ions  Generally Mg2+ is used, but Mn2+ can be utilized for PCR mediated DNA mutagenesis As higher Mn2+ concentration increases the error rate during DNA synthesis
  • 14. 14  PCR, POLYMERASE CHAIN REACTION, is an in-vitro technique that allows amplification of a particular DNA sequence and is able to generate innumerable copies of specific DNA sequence.
  • 15. 15 PRINCIPLE A characteristic feature of DNA is that bringing it to a certain high temperature known as melting temperature (Tm) ↓ The double strands fall apart into single strands by dissolution of the H-bonds ↓ When the temperature is lowered , the two strands again anneal to restore the double helix structure (annealing temperature) ↓ PCR technique utilizes this property of DNA for replication
  • 16. 16 THE PCR MACHINE  The PCR machine is a thermal cycler in which the temperature , time and number of cycles required for amplification of the sample DNA can be preset for automatic operation.  Normal DNA polymerase is thermo labile → a thermo stable DNA polymerase obtained from a thermophilic organism is used.  This avoids the addition of the enzyme in each cyclic operation.
  • 18. 18 THE PCR CYCLE Comprised of 3 steps: • Denaturation of DNA at 950C • Primer hybridization ( annealing) at 40-500C • DNA synthesis ( Primer extension) at 720C
  • 19. 19 DENATURATION The first step is the denaturation of DNA sample in a reaction mixture to 95 °C . At this thermal condition DNA strand gets separated. The temperature is maintained up to 5 minutes.
  • 20. 20 RENATURATION The temperature is lowered to 50 °C to allow the 2 oligonucleotide primers to anneal (bind) to the complementary sequence in the DNA molecule. The time duration of 30 seconds is maintained for renaturation.
  • 21. 21 SYNTHESIS OF NEW DNA The temperature is raised to 72-75 °C . At this elevated temperature , Taq polymerase shows optimum activity and initiates DNA synthesis at 3 hydroxyl end of each primer.
  • 22. 22
  • 23. 23
  • 25. 25 TYPES OF PCR  Several modifications of PCR have been developed for specific applications  Another reason for the modification is to overcome problems or trouble shooters during amplification.  Following are some of the improved version of PCR.  Nested PCR  Inverse PCR  Hot start PCR
  • 26. 26 1. NESTED PCR  Nested PCR is a variation of the polymerase chain reaction , in that 2 pairs ( instead of 1 pair) of PCR primers are used to amplify a fragment. TECHNIQUE Step 1 : primers binds to template DNA and PCR start. Step 2 : PCR products from the first PCR reaction are subjected to a second PCR run. Step 3 : we can get multiple copies
  • 27. 27
  • 28. 28 2. HOT-START PCR A technique that reduces non-specific amplification during the initial set up stages of the PCR. It may be performed manually by heating the reaction components to the melting temperature (eg.95ᵒC) before adding the polymerase.  2 types a. Mechanical hot start b. non-mechanical hot start
  • 29. 29  MECHANICAL HOT START PCR All components of PCR are added to the PCR vial except for the DNA polymerase enzyme which will be added just at the first denaturation step.  NON-MECHANICAL HOT START PCR The use of a form of Taq DNA polymerase , for example , Amplitaq Gold which is activated only if the reaction mixture is heated at about 94ᵒC ( the first denaturation step)
  • 30. 30  Other methods depend on covalent linking of the polymerase enzyme to certain inhibitors. The enzyme becomes dissociated from these inhibitors at the first denaturation step.
  • 31. 31
  • 33. 33 3. INVERSE PCR Target DNA is lightly cut into smaller fragments of several kilobases by restriction endonuclease digestion. Self-ligation is induced under low concentrations causing the phosphate backbone to reform. This gives a circular DNA ligation product. Target DNA is then restriction digested with a known endonuclease.
  • 34. 34 This generates a cut within the known internal sequence generating a linear product with known terminal sequences. This can now be used for PCR (polymerase chain reaction)
  • 36. 36 OTHER VARIATIONS OF THE PCR Colony PCR Multiplex PCR Asymmetric PCR Long PCR Allele specific PCR Real time PCR Reverse transcriptase PCR (RT-PCR) In situ PCR Long accurate PCR Touch down PCR AFLP PCR
  • 37. 37 • Automated, fast, reliable (reproducible) results • High output • Sensitive • Broad uses • Defined, easy to follow protocols • Commercial kits are now available for easy PCR reaction setup and amplification ADVANTAGES
  • 38. 38 DISADVANTAGES • Extreamly liable to contamination • High degree of operator skills required • False positive results due to amplifications • Expensive to the developing world
  • 39. 39 APPLICATIONS • It is extensively used for the amplification of a particular target DNA sequence • Genome mapping and gene function determination • Biodiversity studies ( e.g. evolution studies) • Detection of drug resistance genes • In plant biotechnology, PCR is used in plant disease identification , presence of any target gene in crop plants
  • 40. 40 • The PCR is widely employed in disease diagnosis (early detection of cancer, viral infections...) . • The speed and sensitivity of PCR helps in prenatal diagnosis of inherited disease. • Forensic (DNA fingerprinting) • PCR has an important role in gene manipulation and expression studies.
  • 41. 41 REFERENCE  Biotechnology-4 by S. Mahesh and A.B Vedamurthy , Page number : 32-35  Ananthanarayanan and Paniker’s text book of microbiology , 7th edition. C K J Paniker. Page number : 591  Molecular biology and biotechnology , 5th edition. John M Walker and Ralph Rapley. Page number : 15- 18  www.wikipedia.com
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