Oligo swapping method for in vitro DNA repair substrate containing a single DNA lesion at a specific site

Abstract Background A wide variety of DNA lesions interfere with replication and transcription, leading to mutations and cell death. DNA repair mechanisms act upon these DNA lesions present in the genomic DNA. To investigate a DNA repair mechanism elaborately, an in vitro DNA repair substrate contai...

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Main Authors: Mika Yukutake, Mika Hayashida, Narumi Shioi Aoki, Isao Kuraoka
Format: Article
Language:English
Published: BMC 2018-11-01
Series:Genes and Environment
Subjects:
Online Access:http://link.springer.com/article/10.1186/s41021-018-0112-5
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spelling doaj-b501037c47d749e794dbdbadfe04a5c42020-11-25T03:24:52ZengBMCGenes and Environment1880-70622018-11-014011910.1186/s41021-018-0112-5Oligo swapping method for in vitro DNA repair substrate containing a single DNA lesion at a specific siteMika Yukutake0Mika Hayashida1Narumi Shioi Aoki2Isao Kuraoka3Department of Chemistry, Faculty of Science, Fukuoka UniversityDepartment of Chemistry, Faculty of Science, Fukuoka UniversityDepartment of Chemistry, Faculty of Science, Fukuoka UniversityDepartment of Chemistry, Faculty of Science, Fukuoka UniversityAbstract Background A wide variety of DNA lesions interfere with replication and transcription, leading to mutations and cell death. DNA repair mechanisms act upon these DNA lesions present in the genomic DNA. To investigate a DNA repair mechanism elaborately, an in vitro DNA repair substrate containing DNA lesions at a specific site is required. Previously, to prepare the substrate, phagemid ssDNA and DNA lesion-harboring oligonucleotides were employed with considerable amounts of DNA polymerase and DNA ligase. However, preparing in vitro DNA repair substrate in general is difficult and labor intensive. Results Here, we modified the construction method of in vitro mismatch repair substrate using a nicking-endonuclease, which produces gap corresponding to the ssDNA in the plasmid DNA, and swaps DNA lesion-containing oligonucleotide upon addition of restriction enzyme and T5 exonuclease. This modified method is able to produce in vitro DNA repair substrates containing adenine:cytosine mismatch basepair, 8-oxoG, and uracil. The DNA repair enzyme, each Fpg, hOGG1 could cleave an 8-oxoG-containing DNA substrate, the mixture of UDG and APE1 could cleave a uracil-containing DNA substrate. Omitting a column purification step, DNA repair substrates were prepared by one-pot synthesis. Conclusions We were able to prepare in vitro DNA repair substrates using this simple method involving restriction enzymes and T5 exonuclease. It is anticipated that this method, termed as “Oligo Swapping Method”, will be valuable for understanding the DNA repair machinery.http://link.springer.com/article/10.1186/s41021-018-0112-5DNA lesionIn vitro DNA repair substrateIn vitro assay
collection DOAJ
language English
format Article
sources DOAJ
author Mika Yukutake
Mika Hayashida
Narumi Shioi Aoki
Isao Kuraoka
spellingShingle Mika Yukutake
Mika Hayashida
Narumi Shioi Aoki
Isao Kuraoka
Oligo swapping method for in vitro DNA repair substrate containing a single DNA lesion at a specific site
Genes and Environment
DNA lesion
In vitro DNA repair substrate
In vitro assay
author_facet Mika Yukutake
Mika Hayashida
Narumi Shioi Aoki
Isao Kuraoka
author_sort Mika Yukutake
title Oligo swapping method for in vitro DNA repair substrate containing a single DNA lesion at a specific site
title_short Oligo swapping method for in vitro DNA repair substrate containing a single DNA lesion at a specific site
title_full Oligo swapping method for in vitro DNA repair substrate containing a single DNA lesion at a specific site
title_fullStr Oligo swapping method for in vitro DNA repair substrate containing a single DNA lesion at a specific site
title_full_unstemmed Oligo swapping method for in vitro DNA repair substrate containing a single DNA lesion at a specific site
title_sort oligo swapping method for in vitro dna repair substrate containing a single dna lesion at a specific site
publisher BMC
series Genes and Environment
issn 1880-7062
publishDate 2018-11-01
description Abstract Background A wide variety of DNA lesions interfere with replication and transcription, leading to mutations and cell death. DNA repair mechanisms act upon these DNA lesions present in the genomic DNA. To investigate a DNA repair mechanism elaborately, an in vitro DNA repair substrate containing DNA lesions at a specific site is required. Previously, to prepare the substrate, phagemid ssDNA and DNA lesion-harboring oligonucleotides were employed with considerable amounts of DNA polymerase and DNA ligase. However, preparing in vitro DNA repair substrate in general is difficult and labor intensive. Results Here, we modified the construction method of in vitro mismatch repair substrate using a nicking-endonuclease, which produces gap corresponding to the ssDNA in the plasmid DNA, and swaps DNA lesion-containing oligonucleotide upon addition of restriction enzyme and T5 exonuclease. This modified method is able to produce in vitro DNA repair substrates containing adenine:cytosine mismatch basepair, 8-oxoG, and uracil. The DNA repair enzyme, each Fpg, hOGG1 could cleave an 8-oxoG-containing DNA substrate, the mixture of UDG and APE1 could cleave a uracil-containing DNA substrate. Omitting a column purification step, DNA repair substrates were prepared by one-pot synthesis. Conclusions We were able to prepare in vitro DNA repair substrates using this simple method involving restriction enzymes and T5 exonuclease. It is anticipated that this method, termed as “Oligo Swapping Method”, will be valuable for understanding the DNA repair machinery.
topic DNA lesion
In vitro DNA repair substrate
In vitro assay
url http://link.springer.com/article/10.1186/s41021-018-0112-5
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