2002
DOI: 10.1023/a:1015250426726
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Abstract: A new method for hybridization analysis of nucleic acids is proposed on the basis of the ability of site-specific nickases to cleave only one DNA strand. The method is based on the use of a labeled oligonucleotide with the recognition site of the nickase hybridized with the target (DNA or RNA) at an optimal temperature of the enzyme (55 degrees C). The two shorter oligonucleotides formed after the cleavage with the nickase do not complex with the target. Thus, a multiple cleavage of the labeled oligonucleotide… Show more

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Cited by 16 publications
(10 citation statements)
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“…We have used the ability of nicking endonucleases to cut only one DNA strand in elaboration of a new method of DNA target detection in a reaction proceeding at con stant temperature (55°C) [41,42]. A molecular beacon and a nickase (Nt.BspD6I isolated by us was used in this work) are involved in the reaction.…”
Section: Practical Application Of Nicking Endonucleasesmentioning
confidence: 99%
“…We have used the ability of nicking endonucleases to cut only one DNA strand in elaboration of a new method of DNA target detection in a reaction proceeding at con stant temperature (55°C) [41,42]. A molecular beacon and a nickase (Nt.BspD6I isolated by us was used in this work) are involved in the reaction.…”
Section: Practical Application Of Nicking Endonucleasesmentioning
confidence: 99%
“…The plasmid pRARE/sscL1IM contains the methylase M.SscL1I gene inserted into plasmid pRARE. The M.SscL1I has been shown to protect host DNA against hydrolysis by the nickase (Zheleznaya et al, 2002). The pRARE (Novagen) contains genes of tRNA that rarely occur in E. coli.…”
Section: Expression and Purification Of The Nickasementioning
confidence: 99%
“…Four naturally occurring enzymes have so far been identi®ed in bacterial sources (Abdurashitov et al, 1996;Morgan et al, 2000;Zheleznaya et al, 2002;Dedkov et al, 2001). One of them, the nickase Nb.BspD6I (N.BspD6I in old nomenclature), was found and characterized by Zheleznaya et al (2002). All the enzymes recognize the DNA sequence 5 H -GAGTC-3 H /5 H -GACTC-3 H and cleave only the top strand 4 bp downstream of the recognition site.…”
Section: Introductionmentioning
confidence: 99%
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