Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... ·...

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Ameer Effat M. Elfarash Dept. of Genetics Fac. of Agriculture, Assiut Univ. [email protected] Troubleshooting of Real Time PCR

Transcript of Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... ·...

Page 1: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly

Ameer Effat M. Elfarash

Dept. of Genetics

Fac. of Agriculture, Assiut Univ.

[email protected]

Troubleshooting of Real Time PCR

Page 2: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly

What is Real-Time PCR used for?

• Gene expression analysis

• Disease diagnosis and management

– Viral quantification

• Food testing

– Percent GMO food

• Animal and plant breeding

– Gene copy number

Page 3: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly
Page 4: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly
Page 5: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly
Page 6: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly

Background

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Page 8: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly

PCR itself as a problem

• The PCR reaction • Template concentration

• Inhibitors

• Optimization

• The operator • Pipetting errors

• Setting up reactions

• Wrong PCR programs

Page 9: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly

We describe the position of the lines with a value that represents the cycle number

where the trace crosses a threshold.

This is called the cycle threshold “Ct Value”.

Ct values are directly related to the starting quantity of DNA, by way of the formula:

Quantity = 2^Ct

0

500000

1000000

1500000

2000000

2500000

3000000

3500000

4000000

4500000

5000000

0 5 10 15 20 25 30 35 40

23 25 28

Ct Values:

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Standard curves

• Serial dilutions of known sequences used for ‘metering’ of unknown concentrations

A

B

Who is taller, A or B?

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Ideal Standard Curves

Ct

Log copies

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PCR Efficiency Efficiency reflects whether DNA doubled

every cycle It takes 3.32 cycles for DNA to be amplified

10 fold If samples have been correctly diluted, every

10-fold dilution should be 3.32 cycles

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• Problematic qRT-PCR – No amplification

– Unexpected efficiency

– Delayed Ct

– Scattered replicates

– Unusual curves

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No Amplification

• Missing a master mix component(Repeat the experiment)

• Sample degradation (Do a different cDNA prep - Test a positive control)

• Machine not calibrated for dye (Calibrate the instrument)

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Unexpected PCR Efficiency • Lower efficiency (<85%)

– Incorrect dilutions causing errors in standard curve

– Lower fluorescence of dye

– Instrument not calibrated for dye

– Sample inhibition

Incorrect dilutions

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Unexpected PCR Efficiency

• Higher efficiency (>110%)

– Incorrect dilutions causing errors in standard curve

– Genomic DNA contamination

– Incomplete DNase treatment

– Primers Dimer

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primer dimers

• Primer-dimers interferes with quantitation

• Identifying primer-dimers: melting curve analysis – Pure, homogenous PCR products produce a single, sharply defined

melting curve with a narrow peak. Primer dimers melt at relatively low temperatures and have broader peak

Page 18: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly

5’

5’

3’ 3’

ID ID ID

CO

LD

5’

5’

3’

3’ ID

ME

DIU

M

5’

5’

3’

3’

HO

T

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5’ 5’ 3’ 3’

5’

5’

3’

3’

ID ID ID

5’

5’

3’ 3’ ID

• Melt curves can tell us what products are in a reaction.

• PCR products that are shorter will melt at lower temperatures.

• Different PCR products will therefore have different shaped curves.

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• For convenience, we typically view the derivative (slope) of the actual melt curve data.

• The resulting graph looks like a chromatogram, with peaks that represent different PCR products.

These PCR products

melt at a relatively low temperature, are likely primer-dimers.

These PCR products

melt at a higher temperature, and are likely to be the main

PCR product.

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How to avoid primer/dimers?

• General approaches – Reduce delays in workflow – Optimize primer – Increase the annealing temperature Reduce

annealing time to 1-5 sec. – Use hot start – Reduce number of cycles, e.g. to 40

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Delayed Ct

• Low expression

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Delayed Ct……Sample inhibition

• The concentration of inhibitors is maximum in the least dilute sample

• As the sample is diluted, the inhibitory effect decreases – Make a new cDNA

prep

10-fold dilution

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Inhibitors

• Re-extraction, ethanol precipitation, and/or centrifugal ultrafiltration may correct the problem – chloroform

– SDS concentrations of as low as 0.01% are inhibitory

– phenol

– heparin

– bromphenol blue

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Master Mix A

Master Mix B

Delayed Ct…… Master mixes can make a difference

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Scattered Replicates

• Pipetting errors

• Incorrectly set baseline

Replicates ideally should not be more than 0.5 Ct apart

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Unusual curves……….Sample evaporation

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Unexpected Signal…

• Positive NTC: maybe master mix got contaminated

• Assay design

• Positive –RT -> gDNA contamination

– Incomplete DNase treatment

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• A successful real-time PCR experiment will have the following characteristics:

Replicates are

tightly clustered

Baselines are

relatively flat

Dilution series has

expected spacing

Plateau height

doesn’t matter

Melt curve has one

peak per product.

Curves are all

S-shaped

Curves are

smooth

Page 30: Troubleshooting of Real Time PCR - Assiut University ... of PCR level 2 (5.7-4... · Troubleshooting of Real Time PCR . ... • Gene expression analysis ... Ct values are directly