1. Introduction to Real-Time PCR
Joachim Hegstad
Forsker
Avdeling for Mikrobiologi og Smittevern
Universitetssykehuset Nord-Norge
2. Main Topics What is PCR?
PCR detection methods
Real-Time PCR Instruments
Software analyses
Clinical value
3. Polymerase Chain Reaction (PCR) (1) PCR was invented by Dr. Kary Mullis i 1983 –Nobel price in chemistry ten years later.
PCR is by far one of the most important and used molecular tool in diagnostic and science.
By May 2009, 380 990 paper were published using PCR as a tool (PubMed)
PCR imitate natures way of copying DNA by amplifying DNA sequence specified/limited by the primers.
4. Polymerase Chain Reaction (PCR) (2) PCR mix must contain:
Template (DNA/RNA sample containing the target)
DNA polymerase
Co-factor such as Mg2+
Primers ( 20 – 30 bp)
Deoxyribonucleotides (dATP, dCTP, dGTP, and dTTP)
5. Polymerase Chain Reaction (PCR) (3) The PCR program normally cycles bewteen 3 temperatures which are repeated
Denaturation of DNA 94 – 96°C in = 20 sec.
DNA is denatured to single stranded DNA
Annealing, 50 – 65°C in = 20 sec.
Primers binds to complementary sequence on both target sequences of single stranded DNA
Extention, 72°C in = 20 sec.
Polymerase binds to and incorporate complementary nucleotides from primers and downstream target sequence
6. Detection of PCR product by electrophoresis
PCR product is loaded in wells on agarose gel (0,6-2,5%)
Electrophoresis separates DNA by size
Visualisation in UV-light after staining by EtBr
7. Fluorescence-detection methods
8. SYBER Green detection
9. Double Dye probes TaqMan probe
Doube-Dye LNA probe
MGB probe
10. Molecular Beacons
11. FRET probes or Hybridisation probes�(fluorescence resonance energy transfer)
12. Fluorophores and quenchers (1)
13. Fluorophores and quenchers (2)
14. Real-Time PCR Instruments ABI Prism SDS:
7900 Fast
7500 Fast
7300
7000
Roche
Light Cycler 1.0/2.0
LightCycler® 480
Cepheid
Smart Cycler
BioRad
Icycler iQ5
Stratagene
Mx3005P
Mx3000P
Mx4000
Corbett/Qiagen
Roto-Gene 3000
Rotor-Gene 6000/Qiagen Gene Q
NucliSens MB Analyzer
15. Real-Time PCR Instruments (2)�ABI 7900 Fast 96 or 384 well format
40 cycles in 30 min in 96-Fast-format and 55 min in 384-format
Closed well system
Minimal hands-on
Dynamic range of 6 orders of magnitude
Multi-color detection
Qualitative and quantitative testing
16. Real-Time PCR Instruments (3)�Real-Time PCR Set-up Plastics
Optical 96-well
384-well plates
Tubes (only on 96 cycler)
Reaction volume 96-well < 100 µl
Reaction volume 384-well < 20 µl
Optical adhesive covers or caps
17. Real-Time PCR Instruments (4) �Applied Biosystems Line
18. Real-Time PCR Instruments (5) �Roche Glass capillaries
Air heating and cooling
30-40 cycles in 20-30 min
32 sample carousel
20 µl reactions
19. Real-Time PCR Instruments (6) �Cepheid Smart Cycler
20. Real-Time PCR Instruments (7)
21. Real-Time PCR Instruments (8) Corbett Research/Qiagen
Rotor-Gene 3000
Rotor-Gene 6000/Qiagen Gene Q
BioMerieux
NucliSens Easy Q Analyzer System
22. Recommended dyes combinations for multiplex assays on every thermocycler
24. compatibility
25. Data analyses Baseline: PCR cycle number in which signal is accumulating but beneath the limit of detection level of the instrument.
Threshold: Purpose: find a level of fluorescence where samples can be compared.
Sat in the area where the lines are in parallel and amplification is exponential. Fluorescent signal above threshold is used to calculate cycle threshold (Ct).
Ct : (threshold cycle) is defined as the cycle number at which the fluorescence emission exceeds the fixed threshold. It gives the quantitative relationship between amount template in start reaction and amplified product in exponential phase. (quantitation: mRNA expression or DNA copy no). The fewer cycles it takes to reach detectable fluorescence, the greater initial copy number of target.
Rn: Rn+ is the Rn value of a reaction containing all components (the sample of interest); Rn- is the Rn value detected in NTC (baseline value). ?Rn is the difference between Rn+ and Rn-. It is an indicator of the magnitude of the signal generated by the PCR. It is the ?Rn plotted against cycle numbers that produces the amplification curves and gives the CT value.
26. Software analysis of real time PCR
27. SYBR green-detection with dissociation curve
28. Exponential growth phase = linear part in logarithmic graphic
29. Clinical Value Qualitative (pos/neg) nucleic acid tests are especially valuable for the detection of infectious agents that are:
Unculturable
Present in extremely low quantities
Fastidious or slow-growing
30. Clinical Value (2) Quantitative (viral load) methods are important for monitoring certain chronic infections. These tests allow us to:
monitor therapy
detect the development of drug
resistance
predict disease progression
31. Real time PCR vs PCR and detection by electrophoresis Real time PCR
Software detection
Fast – 30 min -2 hours
96 and 384 well formate
Very suitable for quantification – no end point analysis
Achieves no data on size of ampilfied DNA
PCR machine is rather expensive PCR and electrophoresis
Size determination of amplicon
Time and labour intensive
Few samples per gel
Pour quantification – end point analysis
