Preparation of Phi29 DNA polymerase free of amplifiable DNA using ethidium monoazide, an ultraviolet-free light-emitting diode lamp and trehalose.
We previously reported that multiply-primed rolling circle amplification (MRPCA) using modified random RNA primers can amplify tiny amounts of circular DNA without producing any byproducts. However, contaminating DNA in recombinant Phi29 DNA polymerase adversely affects the outcome of MPRCA, especia...
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Public Library of Science (PLoS)
2014-01-01
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| Series: | PLoS ONE |
| Online Access: | http://europepmc.org/articles/PMC3915000?pdf=render |
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doaj-092298efef7f45ad8df3fcbc5c65e01a2020-11-25T02:22:10ZengPublic Library of Science (PLoS)PLoS ONE1932-62032014-01-0192e8262410.1371/journal.pone.0082624Preparation of Phi29 DNA polymerase free of amplifiable DNA using ethidium monoazide, an ultraviolet-free light-emitting diode lamp and trehalose.Hirokazu TakahashiHiroyuki YamazakiSatoshi AkanumaHiroko KanaharaToshiyuki SaitoTomoyuki ChimuroTakayoshi KobayashiToshio OhtaniKimiko YamamotoShigeru SugiyamaToshiro KoboriWe previously reported that multiply-primed rolling circle amplification (MRPCA) using modified random RNA primers can amplify tiny amounts of circular DNA without producing any byproducts. However, contaminating DNA in recombinant Phi29 DNA polymerase adversely affects the outcome of MPRCA, especially for negative controls such as non-template controls. The amplified DNA in negative control casts doubt on the result of DNA amplification. Since Phi29 DNA polymerase has high affinity for both single-strand and double-stranded DNA, some amount of host DNA will always remain in the recombinant polymerase. Here we describe a procedure for preparing Phi29 DNA polymerase which is essentially free of amplifiable DNA. This procedure is realized by a combination of host DNA removal using appropriate salt concentrations, inactivation of amplifiable DNA using ethidium monoazide, and irradiation with visible light from a light-emitting diode lamp. Any remaining DNA, which likely exists as oligonucleotides captured by the Phi29 DNA polymerase, is degraded by the 3'-5' exonuclease activity of the polymerase itself in the presence of trehalose, used as an anti-aggregation reagent. Phi29 DNA polymerase purified by this procedure has little amplifiable DNA, resulting in reproducible amplification of at least ten copies of plasmid DNA without any byproducts and reducing reaction volume. This procedure could aid the amplification of tiny amounts DNA, thereby providing clear evidence of contamination from laboratory environments, tools and reagents.http://europepmc.org/articles/PMC3915000?pdf=render |
| collection |
DOAJ |
| language |
English |
| format |
Article |
| sources |
DOAJ |
| author |
Hirokazu Takahashi Hiroyuki Yamazaki Satoshi Akanuma Hiroko Kanahara Toshiyuki Saito Tomoyuki Chimuro Takayoshi Kobayashi Toshio Ohtani Kimiko Yamamoto Shigeru Sugiyama Toshiro Kobori |
| spellingShingle |
Hirokazu Takahashi Hiroyuki Yamazaki Satoshi Akanuma Hiroko Kanahara Toshiyuki Saito Tomoyuki Chimuro Takayoshi Kobayashi Toshio Ohtani Kimiko Yamamoto Shigeru Sugiyama Toshiro Kobori Preparation of Phi29 DNA polymerase free of amplifiable DNA using ethidium monoazide, an ultraviolet-free light-emitting diode lamp and trehalose. PLoS ONE |
| author_facet |
Hirokazu Takahashi Hiroyuki Yamazaki Satoshi Akanuma Hiroko Kanahara Toshiyuki Saito Tomoyuki Chimuro Takayoshi Kobayashi Toshio Ohtani Kimiko Yamamoto Shigeru Sugiyama Toshiro Kobori |
| author_sort |
Hirokazu Takahashi |
| title |
Preparation of Phi29 DNA polymerase free of amplifiable DNA using ethidium monoazide, an ultraviolet-free light-emitting diode lamp and trehalose. |
| title_short |
Preparation of Phi29 DNA polymerase free of amplifiable DNA using ethidium monoazide, an ultraviolet-free light-emitting diode lamp and trehalose. |
| title_full |
Preparation of Phi29 DNA polymerase free of amplifiable DNA using ethidium monoazide, an ultraviolet-free light-emitting diode lamp and trehalose. |
| title_fullStr |
Preparation of Phi29 DNA polymerase free of amplifiable DNA using ethidium monoazide, an ultraviolet-free light-emitting diode lamp and trehalose. |
| title_full_unstemmed |
Preparation of Phi29 DNA polymerase free of amplifiable DNA using ethidium monoazide, an ultraviolet-free light-emitting diode lamp and trehalose. |
| title_sort |
preparation of phi29 dna polymerase free of amplifiable dna using ethidium monoazide, an ultraviolet-free light-emitting diode lamp and trehalose. |
| publisher |
Public Library of Science (PLoS) |
| series |
PLoS ONE |
| issn |
1932-6203 |
| publishDate |
2014-01-01 |
| description |
We previously reported that multiply-primed rolling circle amplification (MRPCA) using modified random RNA primers can amplify tiny amounts of circular DNA without producing any byproducts. However, contaminating DNA in recombinant Phi29 DNA polymerase adversely affects the outcome of MPRCA, especially for negative controls such as non-template controls. The amplified DNA in negative control casts doubt on the result of DNA amplification. Since Phi29 DNA polymerase has high affinity for both single-strand and double-stranded DNA, some amount of host DNA will always remain in the recombinant polymerase. Here we describe a procedure for preparing Phi29 DNA polymerase which is essentially free of amplifiable DNA. This procedure is realized by a combination of host DNA removal using appropriate salt concentrations, inactivation of amplifiable DNA using ethidium monoazide, and irradiation with visible light from a light-emitting diode lamp. Any remaining DNA, which likely exists as oligonucleotides captured by the Phi29 DNA polymerase, is degraded by the 3'-5' exonuclease activity of the polymerase itself in the presence of trehalose, used as an anti-aggregation reagent. Phi29 DNA polymerase purified by this procedure has little amplifiable DNA, resulting in reproducible amplification of at least ten copies of plasmid DNA without any byproducts and reducing reaction volume. This procedure could aid the amplification of tiny amounts DNA, thereby providing clear evidence of contamination from laboratory environments, tools and reagents. |
| url |
http://europepmc.org/articles/PMC3915000?pdf=render |
| work_keys_str_mv |
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