Detection of ligation products of DNA linkers with 5'-OH ends by denaturing PAGE silver stain.

Detection of ligation products of DNA linkers with 5'-OH ends by denaturing PAGE silver stain.

To explore if DNA linkers with 5'-hydroxyl (OH) ends could be joined by commercial T4 and E. coli DNA ligase, these linkers were synthesized by using the solid-phase phosphoramidite method and joined by using commercial T4 and E. coli DNA ligases. The ligation products were detected by using de...

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Main Authors: Feng Gao, Huafu Zhou, Wei Li, Xuerong Zhang
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2012-01-01
Series:PLoS ONE
Online Access:http://europepmc.org/articles/PMC3384673?pdf=render
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spelling doaj-512ee1fcec514fd29dd2c25ee34454ae2020-11-24T21:42:19ZengPublic Library of Science (PLoS)PLoS ONE1932-62032012-01-0176e3925110.1371/journal.pone.0039251Detection of ligation products of DNA linkers with 5'-OH ends by denaturing PAGE silver stain.Feng GaoHuafu ZhouWei LiXuerong ZhangTo explore if DNA linkers with 5'-hydroxyl (OH) ends could be joined by commercial T4 and E. coli DNA ligase, these linkers were synthesized by using the solid-phase phosphoramidite method and joined by using commercial T4 and E. coli DNA ligases. The ligation products were detected by using denaturing PAGE silver stain and PCR method. About 0.5-1% of linkers A-B and E-F, and 0.13-0.5% of linkers C-D could be joined by T4 DNA ligases. About 0.25-0.77% of linkers A-B and E-F, and 0.06-0.39% of linkers C-D could be joined by E. coli DNA ligases. A 1-base deletion (-G) and a 5-base deletion (-GGAGC) could be found at the ligation junctions of the linkers. But about 80% of the ligation products purified with a PCR product purification kit did not contain these base deletions, meaning that some linkers had been correctly joined by T4 and E. coli DNA ligases. In addition, about 0.025-0.1% of oligo 11 could be phosphorylated by commercial T4 DNA ligase. The phosphorylation products could be increased when the phosphorylation reaction was extended from 1 hr to 2 hrs. We speculated that perhaps the linkers with 5'-OH ends could be joined by T4 or E. coli DNA ligase in 2 different manners: (i) about 0.025-0.1% of linkers could be phosphorylated by commercial T4 DNA ligase, and then these phosphorylated linkers could be joined to the 3'-OH ends of other linkers; and (ii) the linkers could delete one or more nucleotide(s) at their 5'-ends and thereby generated some 5'-phosphate ends, and then these 5'-phosphate ends could be joined to the 3'-OH ends of other linkers at a low efficiency. Our findings may probably indicate that some DNA nicks with 5'-OH ends can be joined by commercial T4 or E. coli DNA ligase even in the absence of PNK.http://europepmc.org/articles/PMC3384673?pdf=render
collection DOAJ
language English
format Article
sources DOAJ
author Feng Gao
Huafu Zhou
Wei Li
Xuerong Zhang
spellingShingle Feng Gao
Huafu Zhou
Wei Li
Xuerong Zhang
Detection of ligation products of DNA linkers with 5'-OH ends by denaturing PAGE silver stain.
PLoS ONE
author_facet Feng Gao
Huafu Zhou
Wei Li
Xuerong Zhang
author_sort Feng Gao
title Detection of ligation products of DNA linkers with 5'-OH ends by denaturing PAGE silver stain.
title_short Detection of ligation products of DNA linkers with 5'-OH ends by denaturing PAGE silver stain.
title_full Detection of ligation products of DNA linkers with 5'-OH ends by denaturing PAGE silver stain.
title_fullStr Detection of ligation products of DNA linkers with 5'-OH ends by denaturing PAGE silver stain.
title_full_unstemmed Detection of ligation products of DNA linkers with 5'-OH ends by denaturing PAGE silver stain.
title_sort detection of ligation products of dna linkers with 5'-oh ends by denaturing page silver stain.
publisher Public Library of Science (PLoS)
series PLoS ONE
issn 1932-6203
publishDate 2012-01-01
description To explore if DNA linkers with 5'-hydroxyl (OH) ends could be joined by commercial T4 and E. coli DNA ligase, these linkers were synthesized by using the solid-phase phosphoramidite method and joined by using commercial T4 and E. coli DNA ligases. The ligation products were detected by using denaturing PAGE silver stain and PCR method. About 0.5-1% of linkers A-B and E-F, and 0.13-0.5% of linkers C-D could be joined by T4 DNA ligases. About 0.25-0.77% of linkers A-B and E-F, and 0.06-0.39% of linkers C-D could be joined by E. coli DNA ligases. A 1-base deletion (-G) and a 5-base deletion (-GGAGC) could be found at the ligation junctions of the linkers. But about 80% of the ligation products purified with a PCR product purification kit did not contain these base deletions, meaning that some linkers had been correctly joined by T4 and E. coli DNA ligases. In addition, about 0.025-0.1% of oligo 11 could be phosphorylated by commercial T4 DNA ligase. The phosphorylation products could be increased when the phosphorylation reaction was extended from 1 hr to 2 hrs. We speculated that perhaps the linkers with 5'-OH ends could be joined by T4 or E. coli DNA ligase in 2 different manners: (i) about 0.025-0.1% of linkers could be phosphorylated by commercial T4 DNA ligase, and then these phosphorylated linkers could be joined to the 3'-OH ends of other linkers; and (ii) the linkers could delete one or more nucleotide(s) at their 5'-ends and thereby generated some 5'-phosphate ends, and then these 5'-phosphate ends could be joined to the 3'-OH ends of other linkers at a low efficiency. Our findings may probably indicate that some DNA nicks with 5'-OH ends can be joined by commercial T4 or E. coli DNA ligase even in the absence of PNK.
url http://europepmc.org/articles/PMC3384673?pdf=render
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