4.8 Article

MFEprimer-2.0: a fast thermodynamics-based program for checking PCR primer specificity

Journal

NUCLEIC ACIDS RESEARCH
Volume 40, Issue W1, Pages W205-W208

Publisher

OXFORD UNIV PRESS
DOI: 10.1093/nar/gks552

Keywords

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Funding

  1. National Basic Research Project (973 program) [2012CB518200]
  2. Natural Science Foundation of China [30900862, 30973107, 81070741, 81172770]
  3. State Key Laboratory of Proteomics of China [SKLP-O201104, SKLP-K201004, SKLP-O201002]
  4. Special Key Programs for Science and Technology of China [2012ZX09102301-016]

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Evaluating the specificity of polymerase chain reaction (PCR) primers is an essential step in PCR primer design. The MFEprimer-2.0 server allows users to check primer specificity against genomic DNA and messenger RNA/complementary DNA sequence databases quickly and easily. MFEprimer-2.0 uses a k-mer index algorithm to accelerate the search process for primer binding sites and uses thermodynamics to evaluate binding stability between each primer and its DNA template. Several important characteristics, such as the sequence, melting temperature and size of each amplicon, either specific or non-specific, are reported on the results page. Based on these characteristics and the user-friendly output, users can readily draw conclusions about the specificity of PCR primers. Analyses for degenerate primers and multiple PCR primers are also supported in MFEprimer-2.0. In addition, the databases supported by MFEprimer-2.0 are comprehensive, and custom databases can also be supported on request. The MFEprimer-2.0 server does not require a login and is freely available at http://biocompute.bmi.ac.cn/CZlab/MFEprimer-2.0. More over, the MFEprimer-2.0 command-line version and local server version are open source and can be downloaded at https://github.com/quwubin/MFEprimer/wiki/Manual/.

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