Literature DB >> 27222205

Essential strategies to optimize asymmetric PCR conditions as a reliable method to generate large amount of ssDNA aptamers.

Mohammad Heiat1, Reza Ranjbar1, Ali Mohammad Latifi2, Mohammad Javad Rasaee3, Gholamreza Farnoosh2.   

Abstract

Asymmetric PCR, a simple method to generate single-stranded DNA (ssDNA) aptamers in systematic evaluation of ligand by exponential enrichments rounds, is coupled with limitations. We investigated the essential strategies for optimization of conditions to perform a high-quality asymmetric PCR. Final concentrations of primers and template, the number of PCR cycles, and annealing temperature were selected as optimizing variables. The qualities of visualized PCR products were analyzed by ImageJ software. The highest proportion of interested DNA than unwanted products was considered as optimum conditions. Results revealed that the best values for primers ratio, final template concentration, annealing temperature, and PCR cycles were, respectively, 30:1, 1 ng/μL, 55 °C, and 20 cycles for the first and 50:1, 2 ng/μL, 59 °C, and 20 cycles for other rounds. No significant difference was found between optimized asymmetric PCR results in the rounds of two to eight (P > 0.05). The ssDNA quality in round 10 was significantly better than other rounds (P < 0.05). Generally, the ssDNA product with less dimers, double-stranded DNA (dsDNA), and smear are preferable. The dsDNA contamination is the worst, because it can act as antidote and inhibits aptameric performance. Therefore, to choose the best conditions, the lower amount of dsDNA is more important than other unwanted products.
© 2016 International Union of Biochemistry and Molecular Biology, Inc.

Entities:  

Keywords:  asymmetric PCR; optimization; ssDNA aptamer

Mesh:

Substances:

Year:  2017        PMID: 27222205     DOI: 10.1002/bab.1507

Source DB:  PubMed          Journal:  Biotechnol Appl Biochem        ISSN: 0885-4513            Impact factor:   2.431


  17 in total

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Journal:  Front Cell Infect Microbiol       Date:  2022-06-30       Impact factor: 6.073

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6.  Novel Strategies to Optimize the Amplification of Single-Stranded DNA.

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7.  Selection and Identification of Novel Aptamers Specific for Clenbuterol Based on ssDNA Library Immobilized SELEX and Gold Nanoparticles Biosensor.

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Review 8.  Inside the Black Box: What Makes SELEX Better?

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Review 10.  Current and Emerging Methods for the Synthesis of Single-Stranded DNA.

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Journal:  Genes (Basel)       Date:  2020-01-21       Impact factor: 4.096

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