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      An isothermal and sensitive nucleic acids assay by target sequence recycled rolling circle amplification.

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      Biosensors & bioelectronics

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          Abstract

          Sequence-specific nucleic acid detection is playing a more and more important role in modern life sciences. Traditional rolling circle amplification (RCA) involves multiple distinct reaction steps and the experiment result is influenced by multiple factors. What's more, a main limitation of traditional RCA is that each target strand hybridizes with only one padlock probe, and this 1:1 hybridization ratio limits the sensitivity. Here we have proposed target sequence recycled rolling circle amplification (TR-RCA) to increase sensitivity by one step. We demonstrated that our method can not only make RCA occur, but also one target DNA can be reused and thus achieving self-recycle. In TR-RCA, the dumbbell probe recognizes the target DNA and hybridizes with it, and then the stem of the dumbbell probe is opened, after that the opened area anneals with the primer and triggers RCA. At the same time, after a target is displaced, it recognizes and hybridizes with another dumbbell probe, triggering the next cycle of RCA. This amplification method is achievable at a constant temperature simply by mixing dumbbell probes, target DNA, primers, and other chemical complexes together in one tube. Our method has significant advantages in ease of operation. And the results indicate that the target DNA can be detected at fM level with high specificity.

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          Author and article information

          Journal
          Biosens Bioelectron
          Biosensors & bioelectronics
          1873-4235
          0956-5663
          Aug 15 2013
          : 46
          Affiliations
          [1 ] MOE Key Laboratory of Laser Life Science & Institute of Laser Life Science, College of Biophotonics, South China Normal University, Guangzhou 510631, China.
          Article
          S0956-5663(13)00081-X
          10.1016/j.bios.2013.02.003
          23517825
          bfaac9ce-5228-4063-980e-04f0a390ddb1
          Crown Copyright © 2013. Published by Elsevier B.V. All rights reserved.
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