NEB - PCR Protocol Phusion® DNA Polymerase (2024)

Home Protocols PCR Protocol for Phusion^® High-Fidelity DNA Polymerase (M0530)

Overview

The following guidelines are provided to ensure successful PCR using Phusion® DNA Polymerase. These guidelines cover routine PCR. Amplification of templates with high GC content, high secondary structure, low template concentrations or long amplicons may require further optimization.

Protocol

Reaction Setup: We recommend assembling all reaction components on ice and quickly transferring the reactions to a thermocycler preheated to the denaturation temperature (98°C). All components should be mixed and centrifuged prior to use. It is important to add Phusion DNA Polymerase last in order to prevent any primer degradation caused by the 3´→ 5´ exonuclease activity. Phusion DNA Polymerase may be diluted in 1X HF or GC Buffer just prior to use in order to reduce pipetting errors. Please note that protocols with Phusion DNA Polymerase may differ from protocols with other standard polymerases. As such, conditions recommended below should be used for optimal performance.

Component	20 µl Reaction	50 µl Reaction	Final Concentration
Nuclease-free water	to 20 µl	to 50 µl
5X Phusion HF or GC Buffer	4 µl	10 µl	1X
10 mM dNTPs	0.4 µl	1 µl	200 µM
10 µM Forward Primer	1 µl	2.5 µl	0.5 µM
10 µM Reverse Primer	1 µl	2.5 µl	0.5 µM
Template DNA	variable	variable	< 250 ng
DMSO (optional)	(0.6 µl)	(1.5 µl)	3%
Phusion DNA Polymerase	0.2 µl	0.5 µl	1.0 units/50 µl PCR

Notes: Gently mix the reaction. Collect all liquid to the bottom of the tube by a quick spin if necessary. Overlay the sample with mineral oil if using a PCR machine without a heated lid.

Transfer PCR tubes from ice to a PCR machine withthe block preheated to 98°C and begin thermocycling:

Thermocycling conditions for a routine PCR:

STEP	TEMP	TIME
Initial Denaturation	98°C	30 seconds
25-35 Cycles	98°C 45-72°C 72°C	5-10 seconds 10-30 seconds 15-30 seconds per kb
Final Extension	72°C	5-10 minutes
Hold	4-10°C

General Guidelines:

Template:
Use of high quality, purified DNA templates greatly enhances the success of PCR. Recommended amounts of DNA template for a 50 μl reaction are as follows:

DNA	Amount
genomic	50 ng–250 ng
plasmid or viral	1 pg–10 ng

If the template DNA is obtained from a cDNA synthesis reaction, the volume added should be less than 10% of the total reaction volume.

Primers:
Oligonucleotide primers are generally 20–40 nucleotides in length and ideally have a GC content of 40–60%. Computer programs such as Primer3 can be used to design or analyze primers. The final concentration of each primer in a reaction using Phusion DNA Polymerase may be 0.2–1 μM, while 0.5μM is recommended.
Mg⁺⁺ and additives:
Mg⁺⁺is critical to achieve optimal activity with Phusion DNA Polymerase. The final Mg⁺⁺concentration in 1X Phusion HF and GC Buffer is 1.5 mM. Excessive Mg⁺⁺ can prevent full denaturation of DNA as well as cause non-specific binding of primers. The optimal Mg⁺⁺concentration is affected by dNTP concentration, the template being used and supplements that are added to the reaction. This can also be affected by the presence of chelators (e.g. EDTA). Mg⁺⁺can be optimized in 0.5 mM increments using the MgCl₂provided.
Amplification of difficult targets, such as those with GC-rich sequences or secondary structure, may be improved by the presence of additives such as DMSO (included). A final concentration of 3% DMSO is recommended, although concentration can be optimized in 2% increments. It is important to note that if a high concentration of DMSO is used, the annealing temperature must be lowered as it decreases the primer T_m (2). Phusion DNA polymerase is also compatible with other additives such as formamide or glycerol.
Deoxynucleotides:
The final concentration of dNTPs is typically 200 μM of each deoxynucleotide. Phusion cannot incorporate dUTP.
Phusion DNA Polymerase Concentration:
We generally recommend using Phusion DNA Polymerase at a concentration of 20 units/ml (1.0 units/50 μl reaction). However, the optimal concentration of Phusion DNA Polymerase may vary from 10–40 units/ml (0.5–2units/50 μl reaction) depending on amplicon length and difficulty. Do not exceed 2 units/50 µl reaction, especially for amplicons longer than 5 kb.
Buffers:
5X Phusion HF Buffer and 5X Phusion GC Buffer are provided with the enzyme. HF buffer is recommended as the default buffer for high-fidelity amplification. For difficult templates, such as GC-rich templates or those with secondary structure, GC buffer can improve reaction performance. GC buffer should be used in experiments where HF buffer does not work. Detergent-free reaction buffers are also available for applications that do not tolerate detergents (e.g. microarray, DHPLC).
Denaturation:
An initial denaturation of 30 seconds at 98°C is sufficient for most amplicons from pure DNA templates. Longer denaturation times can be used (up to 3 minutes) for templates that require it.
During thermocycling, the denaturation step should be kept to a minimum. Typically, a 5–10 second denaturation at 98°C is recommended for most templates.
Annealing:
Annealing temperatures required for use with Phusion tend to be higher than with other PCR polymerases. The NEB Tm calculatorshould be used to determine the annealing temperature when using Phusion. Typically, primers greater than 20 nucleotides in length anneal for 10–30 seconds at 3°C above the T_m of the lower T_mprimer. If the primer length is less than 20 nucleotides, an annealing temperature equivalent to the T_m of the lower primer should be used. A temperature gradient can also be used to optimize the annealing temperature for each primer pair. For two-step cycling, the gradient can be set as high as the extension temperature.
For high T_mprimer pairs, two-step cycling without a separate annealing step can be used.
Extension:
The recommended extension temperature is 72°C. Extension times are dependent on amplicon length and complexity. Generally, an extension time of 15 seconds per kb can be used. For complex amplicons, such as genomic DNA, an extension time of 30 seconds per kb is recommended. Extension time can be increased to 40 seconds per kb for cDNA templates, if necessary.
Cycle number:
Generally, 25–35 cycles yields sufficient product.
2-step PCR:
When primers with annealing temperatures ≥72°C are used, a 2-step thermocycling protocol is recommended.
Thermocycling conditions for a routine 2-step PCR:

STEP
TEMP
TIME

Initial Denaturation 98°C 30 seconds

25-35 Cycles 98°C
72°C 5-10 seconds
15-30 seconds per kb

Final Extension 72°C 5-10 minutes

Hold 4-10°C
PCR product:
The PCR products generated using Phusion DNA Polymerase have blunt ends; if cloning is the next step, then blunt-end cloning is recommended. If TA-cloning is preferred, then DNA should be purified prior to A-addition, as Phusion DNA Polymerase will degrade any overhangs generated.
Addition of an untemplated -dA can be done with Taq DNA Polymerase (NEB #M0267) or Klenow exo– (NEB #M0212 ).

References:
1. Chester, N. and Marshak, D.R. (1993). Analytical Biochemistry. 209, 284-290.

NEB - PCR Protocol Phusion® DNA Polymerase (2024)

FAQs

How much DNA for PCR phusion? ›

The optimal amount of enzyme depends on the amount of template and the length of the PCR product. Usually 1 unit of Phusion™ High–Fidelity DNA Polymerase per 50 µL reaction volume gives good results, but the optimal amount can range from 0.5 to 2 units per 50 µL reaction depending on amplicon length and difficulty.

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How much DNA is enough for PCR? ›

The recommended amount of DNA template is 25 to 100 ng per 100-µl reaction volume ()pfu polymerase may need ~250 ng genomic DNA), for amplifying single-copy chromosomal targets. Excessively high concentrations of starting DNA can inhibit amplification reactions (> 500-1000 ng).

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How efficient is Phusion DNA polymerase? ›

Better yields with less enzyme Due to their unique structure, Phusion DNA Polymerases are highly efficient and therefore require fewer units per reaction than conventional polymerases. Speed and efficiency result in high product yields in minimal time.

Get More Info Here ›

How accurate is Phusion polymerase? ›

Phusion DNA Polymerase is an ideal choice for cloning and can be used for long or difficult amplicons. With an error rate > 50-fold lower than that of Taq DNA Polymerase and 6-fold lower than that of Pyrococcus furiosus DNA Polymerase (1), Phusion is one of the most accurate thermostable polymerases available.

Can you add too much DNA to PCR? ›

Alter the amount of DNA per reaction.

Too much or too little DNA will result in poor amplification. Run a dilution series of DNA samples including a non-diluted sample, and samples diluted at 1:10, 1:100, and 1:1000 with H2O.

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What is the minimum amount of DNA needed for qPCR? ›

What is the minimum amount of genomic DNA required for analysis using EpiTect Methyl qPCR Arrays? For digestion, we recommend using 0.5-4ug (0.125-1ug per digestion) of genomic DNA for EpiTect Methyl qPCR Arrays and 0.25-0.5ug (0.0625-0.125ug per digestion) for single qPCR assays.

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Can you explain how PCR can detect very low amounts of DNA? ›

PCR tests can detect disease when there is only a very small amount of pathogens in your body. During a PCR test, a small amount of genetic material in a sample is copied multiple times. The copying process is known as amplification. If there are pathogens in the sample, amplification will make them much easier to see.

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What is the expected DNA yield for PCR? ›

The simplest answer is to determine molecular weight of a 1.2 kb DNA and convert that to moles and weight. A 1.2 kb DNA will have a molecular weight of 1200 X 660 grams per mole (6.02 X 10^23 molecules). One DNA fragment will yield 2^30 copies under ideal (100% efficiency) PCR conditions.

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How to calculate DNA concentration for PCR? ›

DNA concentration is estimated by measuring the absorbance at 260nm, adjusting the A₂₆₀ measurement for turbidity (measured by absorbance at 320nm), multiplying by the dilution factor, and using the relationship that an A₂₆₀ of 1.0 = 50µg/ml pure dsDNA.

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Is Q5 better than Phusion? ›

We tested the new Q5 High Fidelity polymerase against Phusion High Fidelity polymerase. The results clearly show a much better yield for Q5 then Phusion. The fragments have been completely sequenced and were devoid of any mistake.

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How fast is Phusion polymerase? ›

High processivity of Phusion Plus DNA NA Polymerase enables amplification of long DNA fragments—up to 10 kb from human gDNA and 20 kb from lambda DNA. Its cycling time is considerably short due to a fast extension rate at 15–30 sec/kb.

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What is the elongation time for PCR Phusion? ›

Generally, an extension time of 15 seconds per kb can be used. For complex amplicons, such as genomic DNA, an extension time of 30 seconds per kb is recommended. Extension time can be increased to 40 seconds per kb for cDNA templates, if necessary.

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What is the error rate of Phusion Taq? ›

For Phusion, the error rate was determined to be 80±39 times better than Taq using the blue/white method and 84 times Taq using the sequencing method. ±= 95% confidence Numbers in brackets have limited statistical significance as only 2 mutations were detected after sequencing 441,670 nucleotides.

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How often does DNA polymerase make a mistake? ›

Nonetheless, these enzymes do make mistakes at a rate of about 1 per every 100,000 nucleotides. That might not seem like much, until you consider how much DNA a cell has. In humans, with our 6 billion base pairs in each diploid cell, that would amount to about 120,000 mistakes every time a cell divides!

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Which DNA polymerase is best for PCR? ›

For this type of routine PCR, you should use a standard thermostable DNA polymerase (like Taq DNA polymerase) to confirm the presence or absence of target DNA. If, however, you are performing cloning experiments or next-generation sequencing (NGS), then accuracy matters.

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How much DNA does PCR yield? ›

PCR can be used to exponentiallyamplify pieces of synthetic DNA flanked by two priming regions, and amplificationsof a single molecule from pools of 1E16 molecules are routinely achieved. Final DNA concentrations ~ 1mg from 0.1 ml reaction volumes are typical,but the yield can vary from 0.1 to 10 mg.

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How much DNA should I use for transfection? ›

The total DNA amount used in calcium phosphate transfection is usually 10–50 μg in 450 μL sterile water and 50 μL of 2.5 M CaCl₂ per 10 cm dish, but varies widely among plasmid preparations as well as with different cells and media.

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How do you calculate DNA volume for PCR? ›

The volume needed can then be calculated as follows: 1.25 Units x (1 µl / 5 Units) = 0.25 µl. The template DNA volume required depends on your sample type.

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How much DNA is needed for lipofectamine? ›

To optimize the amount of Lipofectamine™ 2000 for transfection in a 24-well plate, start with cells at >90% confluency and use a fixed amount of DNA (0.8-1.2 µg). With cell number and DNA concentration held constant, vary the amount of Lipofectamine™ 2000 to determine the optimal concentration (usually 1.5-3 µl).