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HomePolymerase Chain Reaction ApplicationsAmplification of Damaged DNA with Restorase DNA Polymerase

Amplification of Damaged DNA with Restorase DNA Polymerase

Background

Restorase® DNA Polymerase with 10x Reaction Buffer combines Sigma's Long and Accurate enzyme technology with a DNA repair enzyme resulting in a blend that facilitates repair and amplification of damaged DNA. Even though Restorase has been shown to increase yield and specificity of presumably "undamaged" DNA templates, it is not generally recommended to be used in place of standard amplification enzymes on truly undamaged templates.

DNA templates are compromised when damaged by exposure to acid, alkylating agents, heat or light. These damages block the progression of DNA polymerases, thereby affecting PCR efficiency. Restorase functions by modifying the damaged sites allowing subsequent template copying. Restorase can successfully produce PCR products from 0.2 to 20 kb in length.

The level of template damage will dictate optimal Restorase treatment of the DNA. Lightly damaged DNA will require a shorter pretreatment step than templates containing heavier damage. DNA repair begins the moment enzyme is added and ends when the reaction is heated to >50 °C. While Restorase can restore the ability to amplify many damaged DNAs, some templates are irretrievably damaged.

Reagents

  • Restorase® DNA Polymerase with 10x Reaction Buffer (R1028):
    • Restorase DNA Polymerase (L4165)
    • 10 x Restorase Buffer (R8042)
  • PCR grade water (W1754)
  • Primers diluted to working concentration (10µM working stocks are sufficient for most assays)
    • Order Custom Oligos here
  • DNA to be amplified
  • Dedicated pipettes
  • Thermal cycler
  • Sterile filter pipette tips
  • Sterile 1.5 mL screw-top microcentrifuge tubes (such as CLS430909)
  • PCR tubes, select one of the following to match desired format:
  • dNTP mix, 10 mM each of dATP, dCTP, dGTP, and dTTP (D7295, needed for standard format reagents only)

Preparation Instructions

Primer design

It is highly recommended that BigBand™ primers, available from Sigma-Genosys be used in Restorase protocols. These primers are modified to ensure stability during the pre-incubation/repair step. Primer dimer formation during preincubation due to the mesophilic polymerase may be avoided by judicious primer design or manual Primer Hot Start. Primer Hot Start or increased primer concentrations should be used for unmodified primers (see Procedure Step 3 for additional information).

In general, the primers (BigBand or unmodified) are 21 to 34 bases in length and nominally have a GC content of 50%. Melting temperatures (TM) of primer pairs should be within 3 °C of each other and between 60 and 72 °C.1 Primers should also be free of stable secondary structures (e.g. hairpins) or inter/intrahybridization domains that may lead to primer dimer formation. Priming efficiency can be increased by including GC clamps (i.e. 3-prime CC, GG, CG, or GC).2 Using a primer design software is highly recommended.

Template

Restorase is often used to attempt PCR with rare and/or valuable templates that have failed amplifications using standard PCR enzymes. It is prudent to verify thermal cycling conditions using Restorase with easily replenished templates before attempting restorative PCR with irreplaceable templates.

Nicked and/or base damaged DNA can be repaired in most cases. DNA sheared between primer hybridization sites is unrecoverable. Some DNA templates may be damaged beyond repair.

Due to the sources of damaged templates, template quantity is often difficult to measure. Even if the amount of template is known, the extent of damage is likely unknown. For these reasons it is not possible to recommend absolute quantities of template to add to a restorative PCR. In model studies, very lightly depurinated human genomic DNA was successfully amplified from as little as 100 pg while more severe damage required up to 100 ng of template. Thus, for most samples, greater success is realized by using larger quantities (up to 100 ng) of template.

Pre-incubation

Reliable amplification of damaged DNA sequences requires efficient repair and is dependent on the proper pre-incubation time of the reaction. The extent of DNA damage will determine optimal pre-incubation conditions.  

Typical pre-incubation with Restorase is 10 minutes at 37 °C. Lightly damaged DNA will be rescued best by using short incubation times and/or lower temperatures. Heavily damaged DNA may require longer incubation times for optimal rescue.  

If an initial amplification fails, the time of pre-incubation should be investigated to discover an optimal rescue protocol for a particular sample. See Troubleshooting Guide for details on insufficient pre-incubation.

Cycle Number

It is typical that thermal cycling is carried for 30 cycles. In some instances, it may be beneficial to perform additional cycles of PCR. Cycle number optimization may be attempted by performing additional cycles in increments of 5-10 cycles. For damaged DNA samples, it is prudent to withdraw aliquots from the reactions for analysis returning the rest of the reaction for additional cycles. While primer dimer and other primer design artifacts may be magnified by this approach, it may be possible to prepare amplicons that are otherwise missed at lower cycling numbers.

Denaturation

Acid catalyzed depurination is minimized by short denaturation times using Tris buffers pH 9.0 (25 °C) and above. It is recommended that Restorase DNA Polymerase only be used with the supplied magnesium concentration optimized buffer. Follow the protocol below if magnesium optimization is required.

Magnesium concentration

Optimization may be necessary for some template/primer combinations. Magnesium concentration may be optimized by preparing a buffer without magnesium chloride. Magnesium optimization will generally be reached by performing parallel PCR between 1 and 5 mM at 0.5 mM increments (i.e. 1, 1.5, 2 …5 mM).

Buffer preparation

The 10x Restorase Buffer is at a relatively high pH, which may allow precipitation of magnesium hydroxide [Mg(OH)2]. Thaw the buffer at room temperature before use and vigorously vortex to dissolve any precipitated Mg(OH)2 . Alternatively, warm the buffer at 37 °C for 15 minutes and then vortex. Note: It is important that the buffer be homogeneous before reaction assembly.

If titrating pre-incubation times and other PCR optimization experiments fail, it is likely the template is damaged beyond repair and rescue with Restorase.

Storage / Stability

Store Restorase DNA Polymerase and Restorase 10x Buffer at –20 °C.

Procedure

Note: Repair is initiated the moment template and Restorase are mixed. The time between initiation and the initial denaturation step should be tightly controlled.

1.    Add the following reagents to a PCR microcentrifuge tube, strip or plate at ambient temperature:

* Use of BigBand primers, Manual Primer Hot Start, Barrier Primer Hot Start or elevated primer concentration is necessary to minimize the effects of primer degradation by the DNA repair enzyme during pre-incubation. Elevated primer concentrations are dependent upon pre-incubation times. 2 µM is recommended for unprotected primers for 10-minute pre-incubations. Longer pre-incubations require higher primer concentrations, up to 10 µM. Note: If BigBand primers are NOT used, do NOT add primers until after the initial denaturation step.

** Up to 200 ng of template DNA may be necessary for amplification of complex genomes (e.g., human).

***Assumed - Other reaction volumes may be used by scaling this protocol. If a master mix is desired, add template/primers or template to a mix containing buffer, dNTPs and enzyme.

2.    If pre-incubation is less than 3 minutes mix the reaction by re-pipetting after addition of the last reagent (either enzyme or template) at the pre-incubation temperature. Longer pre-incubations may be vortex mixed and briefly centrifuged. Note: Pre-incubation begins the moment enzyme and template are mixed.

3.    Cycling conditions - While amplification parameters may require optimization for specific primers, templates, and thermal cyclers, the protocol below is a good starting point and will suffice in many instances. Note: Pre-incubation time and temperature may be altered depending on the extent of DNA damage (see Pre-incubation under Preparation Instructions).

****Eliminate the Primer Hot Start step above when using BigBand primers.

Primer Hot Start

While paused at the Primer Hot Start step, add 1 µL each of 10 µM forward and reverse primers. The temperature at which primers are added is dependent upon primer design. Primers that yield single product amplicons can be added at low temperatures. Primers that form primer dimer and/or alternate amplicons must be added at elevated temperatures. Resume cycling.

Barrier Primer Hot Start

Add primer solution to HOTSTART® PCR microtubes, Catalog Number H1161- 200 µL or H0911- 500 µL, centrifuge and heat/cool to seal the primers below the wax seal. Add Restorase reaction components and cycle as above.

4.    Evaluate the amplified DNA by standard techniques such as agarose gel electrophoresis.3

Materials
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Troubleshooting Guide

References

1.
Rychlik W, Rhoads RE. 1989. A computer program for choosing optimal oligonudeotides for filter hybridization, sequencing andin vitroamplification of DNA. Nucl Acids Res. 17(21):8543-8551. https://doi.org/10.1093/nar/17.21.8543
2.
Lowe T, Sharefkin J, Yang SQ, Dieffenbach CW. 1990. A computer program for selection of oligonucleotide primers for polymerase chain reactions. Nucl Acids Res. 18(7):1757-1761. https://doi.org/10.1093/nar/18.7.1757
3.
Sambrook J. 2000. Molecular Cloning: A Laboratory Manual. Third Edition. New York: Cold Spring Harbor Laboratory Press.
4.
Don R, Cox PT, Wainwright B, Baker K, Mattick JS. 1991. ?Touchdown? PCR to circumvent spurious priming during gene amplification. Nucl Acids Res. 19(14):4008-4008. https://doi.org/10.1093/nar/19.14.4008
5.
Griffin HG, Griffin AM. 1994. PCR Technology: Current Innovations. Boca Raton, FL: CRC Press.
6.
Innis MA. 1995. PCR Strategies. New York: Academic Press.
7.
Innis M. 1990. PCR Protocols: A Guide to Methods and Applications. San Diego, California: Academic Press.
8.
Newton CR. 1995. PCR: Essential Data Series. New York: John Wiley & Sons.
9.
Roux KH. 1995. Optimization and troubleshooting in PCR.. Genome Research. 4(5):S185-S194. https://doi.org/10.1101/gr.4.5.s185

Label License Statement

NOTICE TO PURCHASER:  LIMITED LICENSE

Use of this product is covered by one or more of the following US patents and corresponding patent claims outside the US:  5,789,224, 5,618,711, 6,127,155 and claims outside the US corresponding to expired US Patent No. 5,079,352. The purchase of this product includes a limited, non-transferable immunity from suit under the foregoing patent claims for using only this amount of product for the purchaser’s own internal research. No right under any other patent claim, no right to perform any patented method, and no right to perform commercial services of any kind, including without limitation reporting the results of purchaser's activities for a fee or other commercial consideration, is conveyed expressly, by implication, or by estoppel. This product is for research use only. Diagnostic uses under Roche patents require a separate license from Roche. Further information on purchasing licenses may be obtained by contacting the Director of Licensing, Applied Biosystems, 850 Lincoln Centre Drive, Foster City, California 94404, USA.

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