2018
DOI: 10.1016/j.ab.2017.12.013
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Blocked recombinase polymerase amplification for mutation analysis of PIK3CA gene

Abstract: A blocked recombinase polymerase amplification (blocked-RPA) approach has been developed for the enrichment of mutated templates in heterogeneous specimens as tumor tissues. This isothermal amplification technique opens alternative solutions for meeting the technological demand of physician office laboratories. Herein, the detection of mutations in PIK3CA gene, such as p.E545K, and p.H1047L, is presented. The main element was an oligonucleotide (dideoxycytidine functionalized at 3'-end) which matched with wild… Show more

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Cited by 27 publications
(33 citation statements)
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“…111,112 In comparison to the heating, proteinase K digestion and SDS treatment methods, usage of the commercial DNA clean-up kit produced only the target band but in a much lower band intensity. 37,109,111 In addition, as an alternative method, centrifugation (3 minutes) to pellet RPA proteins showed equivalent performance to the heating method (65°C for 10 minutes). 110 As with lateral flow strip detection, direct usage of RPA amplicons is possible, but it is recommended to dilute the amplicons with the running buffer (e.g.…”
Section: Amplicon Clean-up and Post-amplification Treatmentmentioning
confidence: 97%
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“…111,112 In comparison to the heating, proteinase K digestion and SDS treatment methods, usage of the commercial DNA clean-up kit produced only the target band but in a much lower band intensity. 37,109,111 In addition, as an alternative method, centrifugation (3 minutes) to pellet RPA proteins showed equivalent performance to the heating method (65°C for 10 minutes). 110 As with lateral flow strip detection, direct usage of RPA amplicons is possible, but it is recommended to dilute the amplicons with the running buffer (e.g.…”
Section: Amplicon Clean-up and Post-amplification Treatmentmentioning
confidence: 97%
“…Most published RPA papers have applied amplicon lengths between 100 and 250 nucleotides, which usually incur fast and efficient amplification. However, shorter amplicons (79 nucleotides; 37 94 nucleotides [38][39][40] and longer amplicon up to 1500 nucleotides 6 and 1941 nucleotides 41 have also been reported. Unlike PCR, the length of RPA primers is relatively long (a recommended minimum of 30 nucleotides, but typically between 32 and 35 nucleotides).…”
Section: Lateral Flow Stripmentioning
confidence: 99%
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“…LAMP has been previously used to detect mutations in tumour tissue such as for KRAS mutations in colorectal colon cancer 32 using LAMP in tandem with ligation substrates. Two studies specific to the detection of PIK3CA mutations published recently involved a colorimetric assay using strand displacement amplification 33 , and recombinase polymerase amplification (RPA), which is another isothermal amplification method 34 . These other studies highlight the demand for a cost-effective and rapid method for mutational tracking of DNA markers in cancer.…”
Section: Discussionmentioning
confidence: 99%