SlideShare a Scribd company logo

Real Time PCR

Download as PPTX, PDF
Bharat Bhushan Negi
Bharat Bhushan Negi

What is PCR ? What is Real Time PCR ? Polymerase Chain Reaction ? What is Reverse Transcriptase Enzyme ? Presented By: Bharat Bhushan Negi M.Tech. Biotechnology IIT Guwahati

Science
1 of 19
Real Time -PCR Bharat Bhushan Negi M.Tech. Biotechnology 174106012 IIT Guwahati (2017-2019)
What is Real Time-PCR ? • Real-Time PCR is a specialized technique that allows a PCR reaction to be visualized “in real time” as the reaction progresses. • This enables researchers to quantify the amount of DNA in the sample at the start of the reaction! • It differs from standard PCR in a way that it can detect the amplified product as the reaction progresses with time but in standard PCR the amplified product is detected at the end of the reaction by agarose gel electrophoresis.
Why Real Time? What's wrong with Agarose Gels ? • End point analysis - End point result is time consuming - End point is variable from sample to sample, while gels may not be able to resolve these variability's in yields. • Low resolution • Low sensitivity • Size-based discrimination only Real-time PCR enables the amount of starting material to be quantified
Real Time Principle • It is based on the detection and quantitation of a fluorescent reporter • In stead of measuring the endpoint we focus on the first significant increase in the amount of PCR product. • If there are only a few DNA molecules at the beginning of the PCR then relatively little product will be made, but if there are many starting molecules then the product yield will be higher.
For Real Time PCR we need a specific probe with a fluorescent reporter
• The probe consists of two types of fluorophores, which are the fluorescent parts of reporter proteins [Green Fluorescent Protein (GFP) has an often- used fluorophore]. • While the probe is attached or unattached to the template DNA and before the polymerase acts, the quencher (Q) fluorophore (usually a long- wavelength colored dye, such as red) reduces the fluorescence from the reporter (R) fluorophore (usually a short-wavelength colored dye, such as green). • It does this by the use of Fluorescence (or Förster) Resonance Energy Transfer (FRET), which is the inhibition of one dye caused by another without emission of a proton. • The reporter dye is found on the 5’ end of the probe and the quencher at the 3’ end. The Taqman probe. The red circle represents the quenching dye that disrupts the observable signal from the reporter dye (green circle) when it is within a short distance
•Once the TaqMan® probe has bound to its specific piece of the template DNA after denaturation (high temperature) and the reaction cools, the primers anneal to the DNA. •Taq polymerase then adds nucleotides and removes the Taqman® probe from the template DNA. •This separates the quencher from the reporter, and allows the reporter to give off its emit its energy. •This is then quantified using a computer. The more times the denaturing and annealing takes place, the more opportunities there are for the Taqman® probe to bind and, in turn, the more emitted light is detected. The TaqMan® probe binds to the target DNA, and the primer binds as well. Because the primer is bound, Taq polymerase can now create a complementary strand.
• The specifications in quantification of the light emitted during real-time PCR are fairly involved and complex The reporter dye is released from the extending double- stranded DNA created by the Taq polymerase. Away from the quenching dye, the light emitted from the reporter dye in an excited state can now be observed.
Other Real Time PCR Methods 1. Molecular Beacon 2. SYBR® Green method •The molecular beacon method utilizes a reporter probe that is wrapped around into a hairpin. It also has a quencher dye that must be in close contact to the reporter to work. •An important difference of the molecular beacon method in comparison to the TaqMan® method is that the probe remains intact throughout the PCR product, and is rebound to the target at every cycle.
This beacon is 33 nucleotides long with a reporter dye attached to the 5' end and a quencher attached to the 3' end. The nine 5' bases are able to form base pairs with the nine 3' bases which brings the reporter and quencher in very close proximity. • Therefore, when the reporter is excited by the appropriate light, its emission is absorbed by the quencher and no fluorescence is detected. • The pink lines represent nucleotides that can form base pairs with the PCR product under investigation.
•As the PCR continues, the newly synthesized PCR products are denatured by high temperatures. •As each strand of the product are separated, the molecular beacon also is denatured so the hairpin structure is disrupted. •As the temperatures cool for the next round of primer annealing, the molecular beacon is capable of forming base pairs with the appropriate strand of the PCR product. • Any molecular beacons that do bind to PCR product reform the hairpin structures and thus are unable to fluoresce. •However, molecular beacons that bind to PCR product remove the ability for the quencher to block fluorescence from the reporter dye. •Therefore, as PCR product accumulates, there is a linear increase in fluorescence.
Detection of PCR product by molecular beacon. •When the beacon binds to the PCR product, it is able to fluoresce when excited by the appropriate wavelength of light. • The amount of fluorescence is directly proportional to the amount of PCR product amplified.
2. SYBR® Green probe method • The SYBR® Green probe was the first to be used in real- time PCR. It binds to double-stranded DNA and emits light when excited. • Unfortunately, it binds to any double-stranded DNA which could result in inaccurate data, especially compared with the specificity found in the other two methods. • Requires extensive optimisation • Longer amplicons create a stronger signal • It´s cheap
How do we carry out PCR if RNA is the starting material? • Real-time PCR is often used to quantify the amount of DNA in an extract • However, this method can be used as a means of measuring RNA amounts, in particular to determine the extent of expression of a particular gene by quantifying its mRNA.
• The first step in this procedure is to convert the RNA molecules into single-stranded complementary DNA (cDNA) using Reverse Transcriptase Enzyme. • Once this preliminary step has been carried out, the PCR primers and Taq polymerase are added and the experiment proceeds exactly as in the standard technique.
Advantages of Real Time PCR • No post-PCR processing of products (high throughput, low contamination risk) • Not influenced by non-specific amplification • Amplification can be monitored real-time • Most specific, sensitive and reproducible
Disadvantages of Real Time PCR • Setting up requires high technical skill and support • High equipment cost • Runs are more expensive than conventional PCR • DNA contamination (in mRNA analysis)
Applications of Real Time PCR • Quantitation of gene expression • Drug therapy efficacy / drug monitoring • Viral quantitation • Pathogen detection
References: 1. IIT Kharagpur- Classroom lecture of Recombinant DNA Technology (PCR) 2. Gene cloning and DNA analysis by T.A Brown 3. NPTEL – Proteomics and Genomics by Dr. Vikash Kumar Dubey (IIT Guwahati) 4. PCR - Applied Biosystem

Recommended

Real time pcr
Real time pcrReal time pcr
Real time pcr
MUSKANKr
 
Real time PCR
Real time PCRReal time PCR
Real time PCR
naren
 
Real time pcr
Real time pcrReal time pcr
Real time pcr
Ibrahim khidir ibrahim osman
 
Nested pcr
Nested pcrNested pcr
Nested pcr
Hritikasinha1
 
Real time PCR
Real time PCRReal time PCR
Real time PCR
Pratyay Seth
 
Rt pcr
Rt pcrRt pcr
Rt pcr
Crimson College of Technology (Pokhara University)
 
Real Time PCR
Real Time PCRReal Time PCR
Real Time PCR
ASHIKH SEETHY
 
Pcr and its types
Pcr and its typesPcr and its types
Pcr and its types
nirvarna gr
 

Recommended

Real time pcr
Real time pcrReal time pcr
Real time pcr
MUSKANKr
 
Real time PCR
Real time PCRReal time PCR
Real time PCR
naren
 
Real time pcr
Real time pcrReal time pcr
Real time pcr
Ibrahim khidir ibrahim osman
 
Nested pcr
Nested pcrNested pcr
Nested pcr
Hritikasinha1
 
Real time PCR
Real time PCRReal time PCR
Real time PCR
Pratyay Seth
 
Rt pcr
Rt pcrRt pcr
Rt pcr
Crimson College of Technology (Pokhara University)
 
Real Time PCR
Real Time PCRReal Time PCR
Real Time PCR
ASHIKH SEETHY
 
Pcr and its types
Pcr and its typesPcr and its types
Pcr and its types
nirvarna gr
 
Polymerase Chain Reaction
Polymerase Chain ReactionPolymerase Chain Reaction
Polymerase Chain Reaction
sara_abudahab
 
Introduction of RT PCR
Introduction of RT PCRIntroduction of RT PCR
Introduction of RT PCR
Md. Shabab Mehebub
 
PCR, Real Time PCR
PCR, Real Time PCRPCR, Real Time PCR
PCR, Real Time PCR
dineshnbagr
 
qRT PCR
qRT PCRqRT PCR
qRT PCR
_mk_ saini
 
Reverse transcriptase polymerase chain reaction
Reverse transcriptase polymerase chain reactionReverse transcriptase polymerase chain reaction
Reverse transcriptase polymerase chain reaction
Vidhi Doshi
 
PCR, RT-PCR and qPCR
PCR, RT-PCR and qPCRPCR, RT-PCR and qPCR
PCR, RT-PCR and qPCR
All India Institute of Medical Sciences
 
PCR Methods and applications
PCR Methods and applicationsPCR Methods and applications
PCR Methods and applications
Behzad Milani
 
Different pcr techniques and their application
Different pcr techniques and their applicationDifferent pcr techniques and their application
Different pcr techniques and their application
saurabh Pandey.Saurabh784
 
Real Time PCR
Real Time PCRReal Time PCR
Real Time PCR
ASHIKH SEETHY
 
Polymerase chain reaction principles and practice
Polymerase chain reaction principles and practice Polymerase chain reaction principles and practice
Polymerase chain reaction principles and practice
subramaniam sethupathy
 
RT PCR
RT PCRRT PCR
RT PCR
mah neem mah
 
Polymerase Chain Reaction - PCR
Polymerase Chain Reaction - PCRPolymerase Chain Reaction - PCR
Polymerase Chain Reaction - PCR
Ahmad Qudah
 
Rt pcr (Reverse transcription PCR)
Rt pcr (Reverse transcription PCR)Rt pcr (Reverse transcription PCR)
Rt pcr (Reverse transcription PCR)
Iqra Wazir
 
Types of PCR
Types of PCRTypes of PCR
Types of PCR
Microbiology
 
Types of PCR
Types of PCRTypes of PCR
Types of PCR
KAUSHAL SAHU
 
Real -Time PCR.pptx
Real -Time PCR.pptxReal -Time PCR.pptx
Real -Time PCR.pptx
ARVINDPRAJAPATI41
 
Multiplex PCR and its Applications
Multiplex PCR and its ApplicationsMultiplex PCR and its Applications
Multiplex PCR and its Applications
Nagendra P
 
MICROARRAY
MICROARRAYMICROARRAY
MICROARRAY
Sanjay Sinhmar
 
Labelling of dna
Labelling of dnaLabelling of dna
Labelling of dna
christanantony
 
Pcr
PcrPcr
Pcr
Tapeshwar Yadav
 
Real time pcr for gene regulation
Real time pcr for gene regulationReal time pcr for gene regulation
Real time pcr for gene regulation
SkAzizuddin1
 
Real-Time PCR
Real-Time PCRReal-Time PCR
Real-Time PCR
Atai Rabby
 

More Related Content

What's hot

What's hot (20)

Polymerase Chain Reaction
Polymerase Chain ReactionPolymerase Chain Reaction
Polymerase Chain Reaction
 
Introduction of RT PCR
Introduction of RT PCRIntroduction of RT PCR
Introduction of RT PCR
 
PCR, Real Time PCR
PCR, Real Time PCRPCR, Real Time PCR
PCR, Real Time PCR
 
qRT PCR
qRT PCRqRT PCR
qRT PCR
 
Reverse transcriptase polymerase chain reaction
Reverse transcriptase polymerase chain reactionReverse transcriptase polymerase chain reaction
Reverse transcriptase polymerase chain reaction
 
PCR, RT-PCR and qPCR
PCR, RT-PCR and qPCRPCR, RT-PCR and qPCR
PCR, RT-PCR and qPCR
 
PCR Methods and applications
PCR Methods and applicationsPCR Methods and applications
PCR Methods and applications
 
Different pcr techniques and their application
Different pcr techniques and their applicationDifferent pcr techniques and their application
Different pcr techniques and their application
 
Real Time PCR
Real Time PCRReal Time PCR
Real Time PCR
 
Polymerase chain reaction principles and practice
Polymerase chain reaction principles and practice Polymerase chain reaction principles and practice
Polymerase chain reaction principles and practice
 
RT PCR
RT PCRRT PCR
RT PCR
 
Polymerase Chain Reaction - PCR
Polymerase Chain Reaction - PCRPolymerase Chain Reaction - PCR
Polymerase Chain Reaction - PCR
 
Rt pcr (Reverse transcription PCR)
Rt pcr (Reverse transcription PCR)Rt pcr (Reverse transcription PCR)
Rt pcr (Reverse transcription PCR)
 
Types of PCR
Types of PCRTypes of PCR
Types of PCR
 
Types of PCR
Types of PCRTypes of PCR
Types of PCR
 
Real -Time PCR.pptx
Real -Time PCR.pptxReal -Time PCR.pptx
Real -Time PCR.pptx
 
Multiplex PCR and its Applications
Multiplex PCR and its ApplicationsMultiplex PCR and its Applications
Multiplex PCR and its Applications
 
MICROARRAY
MICROARRAYMICROARRAY
MICROARRAY
 
Labelling of dna
Labelling of dnaLabelling of dna
Labelling of dna
 
Pcr
PcrPcr
Pcr
 

Similar to Real Time PCR

Real-time polymerase chain reaction.pptx
Real-time polymerase chain reaction.pptxReal-time polymerase chain reaction.pptx
Real-time polymerase chain reaction.pptx
NikitaBankoti2
 
REAL-TIME PCR.pptx by UMNA FATIMA- BIOMED
REAL-TIME PCR.pptx by UMNA FATIMA- BIOMEDREAL-TIME PCR.pptx by UMNA FATIMA- BIOMED
REAL-TIME PCR.pptx by UMNA FATIMA- BIOMED
umnajmi123
 

Similar to Real Time PCR (20)

Real time pcr for gene regulation
Real time pcr for gene regulationReal time pcr for gene regulation
Real time pcr for gene regulation
 
Real-Time PCR
Real-Time PCRReal-Time PCR
Real-Time PCR
 
Types of pcr
Types of pcrTypes of pcr
Types of pcr
 
Real-time polymerase chain reaction.pptx
Real-time polymerase chain reaction.pptxReal-time polymerase chain reaction.pptx
Real-time polymerase chain reaction.pptx
 
Rt pcr
Rt pcrRt pcr
Rt pcr
 
REAL-TIME PCR.pptx by UMNA FATIMA- BIOMED
REAL-TIME PCR.pptx by UMNA FATIMA- BIOMEDREAL-TIME PCR.pptx by UMNA FATIMA- BIOMED
REAL-TIME PCR.pptx by UMNA FATIMA- BIOMED
 
RT-PCR
RT-PCRRT-PCR
RT-PCR
 
Real time PCR.pptx
Real time PCR.pptxReal time PCR.pptx
Real time PCR.pptx
 
Lecture 2 , mbbs students. pcr, rt pcr,
Lecture 2 , mbbs students. pcr, rt pcr, Lecture 2 , mbbs students. pcr, rt pcr,
Lecture 2 , mbbs students. pcr, rt pcr,
 
qRT-PCR.pdf
qRT-PCR.pdfqRT-PCR.pdf
qRT-PCR.pdf
 
TYPES_OF_PCR.pptx
TYPES_OF_PCR.pptxTYPES_OF_PCR.pptx
TYPES_OF_PCR.pptx
 
Real time pcr final
Real time pcr finalReal time pcr final
Real time pcr final
 
Real time pcr
Real time pcrReal time pcr
Real time pcr
 
Real-Time PCR.pptx
Real-Time PCR.pptxReal-Time PCR.pptx
Real-Time PCR.pptx
 
Real time PCR
Real time PCRReal time PCR
Real time PCR
 
real time quantitative pcr
real time quantitative pcr real time quantitative pcr
real time quantitative pcr
 
NIDA FATIMA REAL TIME PCR PPT.pptx
NIDA FATIMA REAL TIME PCR PPT.pptxNIDA FATIMA REAL TIME PCR PPT.pptx
NIDA FATIMA REAL TIME PCR PPT.pptx
 
PCR ,PCR INSTRUMENTATION,STUDYS FOR GENE REGULATION.pptx
PCR ,PCR INSTRUMENTATION,STUDYS FOR GENE REGULATION.pptxPCR ,PCR INSTRUMENTATION,STUDYS FOR GENE REGULATION.pptx
PCR ,PCR INSTRUMENTATION,STUDYS FOR GENE REGULATION.pptx
 
PCR and primer design techniques
PCR and primer design techniquesPCR and primer design techniques
PCR and primer design techniques
 
Real time pcr method
Real time pcr methodReal time pcr method
Real time pcr method
 

Recently uploaded

❤Jammu Kashmir Call Girls 8617697112 Personal Whatsapp Number 💦✅.
❤Jammu Kashmir Call Girls 8617697112 Personal Whatsapp Number 💦✅.❤Jammu Kashmir Call Girls 8617697112 Personal Whatsapp Number 💦✅.
❤Jammu Kashmir Call Girls 8617697112 Personal Whatsapp Number 💦✅.
Nitya salvi
 
Pests of cotton_Borer_Pests_Binomics_Dr.UPR.pdf
Pests of cotton_Borer_Pests_Binomics_Dr.UPR.pdfPests of cotton_Borer_Pests_Binomics_Dr.UPR.pdf
Pests of cotton_Borer_Pests_Binomics_Dr.UPR.pdf
PirithiRaju
 
9999266834 Call Girls In Noida Sector 22 (Delhi) Call Girl Service
9999266834 Call Girls In Noida Sector 22 (Delhi) Call Girl Service9999266834 Call Girls In Noida Sector 22 (Delhi) Call Girl Service
9999266834 Call Girls In Noida Sector 22 (Delhi) Call Girl Service
nishacall1
 
Asymmetry in the atmosphere of the ultra-hot Jupiter WASP-76 b
Asymmetry in the atmosphere of the ultra-hot Jupiter WASP-76 bAsymmetry in the atmosphere of the ultra-hot Jupiter WASP-76 b
Asymmetry in the atmosphere of the ultra-hot Jupiter WASP-76 b
Sérgio Sacani
 
Conjugation, transduction and transformation
Conjugation, transduction and transformationConjugation, transduction and transformation
Conjugation, transduction and transformation
Areesha Ahmad
 
Chemical Tests; flame test, positive and negative ions test Edexcel Internati...
Chemical Tests; flame test, positive and negative ions test Edexcel Internati...Chemical Tests; flame test, positive and negative ions test Edexcel Internati...
Chemical Tests; flame test, positive and negative ions test Edexcel Internati...
ssuser79fe74
 
Discovery of an Accretion Streamer and a Slow Wide-angle Outflow around FUOri...
Discovery of an Accretion Streamer and a Slow Wide-angle Outflow around FUOri...Discovery of an Accretion Streamer and a Slow Wide-angle Outflow around FUOri...
Discovery of an Accretion Streamer and a Slow Wide-angle Outflow around FUOri...
Sérgio Sacani
 
Presentation Vikram Lander by Vedansh Gupta.pptx
Presentation Vikram Lander by Vedansh Gupta.pptxPresentation Vikram Lander by Vedansh Gupta.pptx
Presentation Vikram Lander by Vedansh Gupta.pptx
gindu3009
 

Recently uploaded (20)

Hire 💕 9907093804 Hooghly Call Girls Service Call Girls Agency
Hire 💕 9907093804 Hooghly Call Girls Service Call Girls AgencyHire 💕 9907093804 Hooghly Call Girls Service Call Girls Agency
Hire 💕 9907093804 Hooghly Call Girls Service Call Girls Agency
 
module for grade 9 for distance learning
module for grade 9 for distance learningmodule for grade 9 for distance learning
module for grade 9 for distance learning
 
❤Jammu Kashmir Call Girls 8617697112 Personal Whatsapp Number 💦✅.
❤Jammu Kashmir Call Girls 8617697112 Personal Whatsapp Number 💦✅.❤Jammu Kashmir Call Girls 8617697112 Personal Whatsapp Number 💦✅.
❤Jammu Kashmir Call Girls 8617697112 Personal Whatsapp Number 💦✅.
 
GBSN - Microbiology (Unit 1)
GBSN - Microbiology (Unit 1)GBSN - Microbiology (Unit 1)
GBSN - Microbiology (Unit 1)
 
Pests of cotton_Borer_Pests_Binomics_Dr.UPR.pdf
Pests of cotton_Borer_Pests_Binomics_Dr.UPR.pdfPests of cotton_Borer_Pests_Binomics_Dr.UPR.pdf
Pests of cotton_Borer_Pests_Binomics_Dr.UPR.pdf
 
GBSN - Biochemistry (Unit 1)
GBSN - Biochemistry (Unit 1)GBSN - Biochemistry (Unit 1)
GBSN - Biochemistry (Unit 1)
 
Factory Acceptance Test( FAT).pptx .
Factory Acceptance Test( FAT).pptx .Factory Acceptance Test( FAT).pptx .
Factory Acceptance Test( FAT).pptx .
 
9999266834 Call Girls In Noida Sector 22 (Delhi) Call Girl Service
9999266834 Call Girls In Noida Sector 22 (Delhi) Call Girl Service9999266834 Call Girls In Noida Sector 22 (Delhi) Call Girl Service
9999266834 Call Girls In Noida Sector 22 (Delhi) Call Girl Service
 
GBSN - Microbiology (Unit 2)
GBSN - Microbiology (Unit 2)GBSN - Microbiology (Unit 2)
GBSN - Microbiology (Unit 2)
 
High Class Escorts in Hyderabad ₹7.5k Pick Up & Drop With Cash Payment 969456...
High Class Escorts in Hyderabad ₹7.5k Pick Up & Drop With Cash Payment 969456...High Class Escorts in Hyderabad ₹7.5k Pick Up & Drop With Cash Payment 969456...
High Class Escorts in Hyderabad ₹7.5k Pick Up & Drop With Cash Payment 969456...
 
Feature-aligned N-BEATS with Sinkhorn divergence (ICLR '24)
Feature-aligned N-BEATS with Sinkhorn divergence (ICLR '24)Feature-aligned N-BEATS with Sinkhorn divergence (ICLR '24)
Feature-aligned N-BEATS with Sinkhorn divergence (ICLR '24)
 
Pulmonary drug delivery system M.pharm -2nd sem P'ceutics
Pulmonary drug delivery system M.pharm -2nd sem P'ceuticsPulmonary drug delivery system M.pharm -2nd sem P'ceutics
Pulmonary drug delivery system M.pharm -2nd sem P'ceutics
 
Asymmetry in the atmosphere of the ultra-hot Jupiter WASP-76 b
Asymmetry in the atmosphere of the ultra-hot Jupiter WASP-76 bAsymmetry in the atmosphere of the ultra-hot Jupiter WASP-76 b
Asymmetry in the atmosphere of the ultra-hot Jupiter WASP-76 b
 
Conjugation, transduction and transformation
Conjugation, transduction and transformationConjugation, transduction and transformation
Conjugation, transduction and transformation
 
FAIRSpectra - Enabling the FAIRification of Spectroscopy and Spectrometry
FAIRSpectra - Enabling the FAIRification of Spectroscopy and SpectrometryFAIRSpectra - Enabling the FAIRification of Spectroscopy and Spectrometry
FAIRSpectra - Enabling the FAIRification of Spectroscopy and Spectrometry
 
Proteomics: types, protein profiling steps etc.
Proteomics: types, protein profiling steps etc.Proteomics: types, protein profiling steps etc.
Proteomics: types, protein profiling steps etc.
 
Chemical Tests; flame test, positive and negative ions test Edexcel Internati...
Chemical Tests; flame test, positive and negative ions test Edexcel Internati...Chemical Tests; flame test, positive and negative ions test Edexcel Internati...
Chemical Tests; flame test, positive and negative ions test Edexcel Internati...
 
Discovery of an Accretion Streamer and a Slow Wide-angle Outflow around FUOri...
Discovery of an Accretion Streamer and a Slow Wide-angle Outflow around FUOri...Discovery of an Accretion Streamer and a Slow Wide-angle Outflow around FUOri...
Discovery of an Accretion Streamer and a Slow Wide-angle Outflow around FUOri...
 
Zoology 4th semester series (krishna).pdf
Zoology 4th semester series (krishna).pdfZoology 4th semester series (krishna).pdf
Zoology 4th semester series (krishna).pdf
 
Presentation Vikram Lander by Vedansh Gupta.pptx
Presentation Vikram Lander by Vedansh Gupta.pptxPresentation Vikram Lander by Vedansh Gupta.pptx
Presentation Vikram Lander by Vedansh Gupta.pptx
 

Real Time PCR

  • 1. Real Time -PCR Bharat Bhushan Negi M.Tech. Biotechnology 174106012 IIT Guwahati (2017-2019)
  • 2. What is Real Time-PCR ? • Real-Time PCR is a specialized technique that allows a PCR reaction to be visualized “in real time” as the reaction progresses. • This enables researchers to quantify the amount of DNA in the sample at the start of the reaction! • It differs from standard PCR in a way that it can detect the amplified product as the reaction progresses with time but in standard PCR the amplified product is detected at the end of the reaction by agarose gel electrophoresis.
  • 3. Why Real Time? What's wrong with Agarose Gels ? • End point analysis - End point result is time consuming - End point is variable from sample to sample, while gels may not be able to resolve these variability's in yields. • Low resolution • Low sensitivity • Size-based discrimination only Real-time PCR enables the amount of starting material to be quantified
  • 4. Real Time Principle • It is based on the detection and quantitation of a fluorescent reporter • In stead of measuring the endpoint we focus on the first significant increase in the amount of PCR product. • If there are only a few DNA molecules at the beginning of the PCR then relatively little product will be made, but if there are many starting molecules then the product yield will be higher.
  • 5. For Real Time PCR we need a specific probe with a fluorescent reporter
  • 6. • The probe consists of two types of fluorophores, which are the fluorescent parts of reporter proteins [Green Fluorescent Protein (GFP) has an often- used fluorophore]. • While the probe is attached or unattached to the template DNA and before the polymerase acts, the quencher (Q) fluorophore (usually a long- wavelength colored dye, such as red) reduces the fluorescence from the reporter (R) fluorophore (usually a short-wavelength colored dye, such as green). • It does this by the use of Fluorescence (or Förster) Resonance Energy Transfer (FRET), which is the inhibition of one dye caused by another without emission of a proton. • The reporter dye is found on the 5’ end of the probe and the quencher at the 3’ end. The Taqman probe. The red circle represents the quenching dye that disrupts the observable signal from the reporter dye (green circle) when it is within a short distance
  • 7. •Once the TaqMan® probe has bound to its specific piece of the template DNA after denaturation (high temperature) and the reaction cools, the primers anneal to the DNA. •Taq polymerase then adds nucleotides and removes the Taqman® probe from the template DNA. •This separates the quencher from the reporter, and allows the reporter to give off its emit its energy. •This is then quantified using a computer. The more times the denaturing and annealing takes place, the more opportunities there are for the Taqman® probe to bind and, in turn, the more emitted light is detected. The TaqMan® probe binds to the target DNA, and the primer binds as well. Because the primer is bound, Taq polymerase can now create a complementary strand.
  • 8. • The specifications in quantification of the light emitted during real-time PCR are fairly involved and complex The reporter dye is released from the extending double- stranded DNA created by the Taq polymerase. Away from the quenching dye, the light emitted from the reporter dye in an excited state can now be observed.
  • 9. Other Real Time PCR Methods 1. Molecular Beacon 2. SYBR® Green method •The molecular beacon method utilizes a reporter probe that is wrapped around into a hairpin. It also has a quencher dye that must be in close contact to the reporter to work. •An important difference of the molecular beacon method in comparison to the TaqMan® method is that the probe remains intact throughout the PCR product, and is rebound to the target at every cycle.
  • 10. This beacon is 33 nucleotides long with a reporter dye attached to the 5' end and a quencher attached to the 3' end. The nine 5' bases are able to form base pairs with the nine 3' bases which brings the reporter and quencher in very close proximity. • Therefore, when the reporter is excited by the appropriate light, its emission is absorbed by the quencher and no fluorescence is detected. • The pink lines represent nucleotides that can form base pairs with the PCR product under investigation.
  • 11. •As the PCR continues, the newly synthesized PCR products are denatured by high temperatures. •As each strand of the product are separated, the molecular beacon also is denatured so the hairpin structure is disrupted. •As the temperatures cool for the next round of primer annealing, the molecular beacon is capable of forming base pairs with the appropriate strand of the PCR product. • Any molecular beacons that do bind to PCR product reform the hairpin structures and thus are unable to fluoresce. •However, molecular beacons that bind to PCR product remove the ability for the quencher to block fluorescence from the reporter dye. •Therefore, as PCR product accumulates, there is a linear increase in fluorescence.
  • 12. Detection of PCR product by molecular beacon. •When the beacon binds to the PCR product, it is able to fluoresce when excited by the appropriate wavelength of light. • The amount of fluorescence is directly proportional to the amount of PCR product amplified.
  • 13. 2. SYBR® Green probe method • The SYBR® Green probe was the first to be used in real- time PCR. It binds to double-stranded DNA and emits light when excited. • Unfortunately, it binds to any double-stranded DNA which could result in inaccurate data, especially compared with the specificity found in the other two methods. • Requires extensive optimisation • Longer amplicons create a stronger signal • It´s cheap
  • 14. How do we carry out PCR if RNA is the starting material? • Real-time PCR is often used to quantify the amount of DNA in an extract • However, this method can be used as a means of measuring RNA amounts, in particular to determine the extent of expression of a particular gene by quantifying its mRNA.
  • 15. • The first step in this procedure is to convert the RNA molecules into single-stranded complementary DNA (cDNA) using Reverse Transcriptase Enzyme. • Once this preliminary step has been carried out, the PCR primers and Taq polymerase are added and the experiment proceeds exactly as in the standard technique.
  • 16. Advantages of Real Time PCR • No post-PCR processing of products (high throughput, low contamination risk) • Not influenced by non-specific amplification • Amplification can be monitored real-time • Most specific, sensitive and reproducible
  • 17. Disadvantages of Real Time PCR • Setting up requires high technical skill and support • High equipment cost • Runs are more expensive than conventional PCR • DNA contamination (in mRNA analysis)
  • 18. Applications of Real Time PCR • Quantitation of gene expression • Drug therapy efficacy / drug monitoring • Viral quantitation • Pathogen detection
  • 19. References: 1. IIT Kharagpur- Classroom lecture of Recombinant DNA Technology (PCR) 2. Gene cloning and DNA analysis by T.A Brown 3. NPTEL – Proteomics and Genomics by Dr. Vikash Kumar Dubey (IIT Guwahati) 4. PCR - Applied Biosystem