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    Single nucleotide polymorphism-mismatch primer development for rapid molecular identification of selected microalgal species

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    Park_et_al_2021.pdf
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    Description:
    Final Accepted Manuscript
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    Author
    Park, Sang-Hyuck
    Steichen, Seth Alan
    Brown, Judith K.
    Affiliation
    School of Plant Sciences, The University of Arizona
    Issue Date
    2021-02-24
    Keywords
    Microalgae
    Molecular diagnostics
    Quality control
    Single nucleotide polymorphism
    
    Metadata
    Show full item record
    Publisher
    Springer Science and Business Media LLC
    Citation
    Park, SH., Steichen, S.A. & Brown, J.K. Single nucleotide polymorphism-mismatch primer development for rapid molecular identification of selected microalgal species. J Appl Phycol (2021).
    Journal
    Journal of Applied Phycology
    Rights
    © The Author(s), under exclusive licence to Springer Nature B.V. part of Springer Nature 2021.
    Collection Information
    This item from the UA Faculty Publications collection is made available by the University of Arizona with support from the University of Arizona Libraries. If you have questions, please contact us at repository@u.library.arizona.edu.
    Abstract
    Microalgae have been a great source for food, cosmetic, pharmacological, and biofuel production. The adoption of effective diagnostic assays for monitoring all stages of algal cultivation has become essential. In addition to microscopy identification, molecular assays can aid greatly in the identification and monitoring of algal species of interest. In this study the 18S ribosomal RNA (rRNA) sequences of 12 microalgal species and/or strains were used to design algal identification primers. Sequence alignment revealed five highly variable regions and multiple unique single nucleotide polymorphisms (SNPs). To design target algae specific primers, a SNP identified as unique to each microalgal species was incorporated into the 3’-terminus of forward and reverse primer pairs, respectively. To further enhance primer specificity, transverse mutation was introduced into each primer at the third base upstream of the respective SNP. The SNP-mismatch primer pairs yield size-specific amplicons, enabling the rapid molecular detection of 12 microalgae by circumventing cloning and sequencing. To verify the primer specificity, two SNP-mismatch primer pairs designed for Chlorella sorokiniana DOE1412 and wildtype species of Scenedesmus were tested in the outdoor reactor run inoculated with C. sorokiniana DOE1412. The primer pairs were able to identify C. sorokiniana DOE1412 as well as the environmental invader Scenedesmus sp. Furthermore, the “relative concentration” of two microalgae was accessed throughout the entire cultivation run. The use of SNPs primers designed in this study offers a cost-effective, easy to use alternative for routine monitoring of microalgal cultures in laboratories, in scale-ups, and in cultivation reactors, independent of the production platform. © 2021, The Author(s), under exclusive licence to Springer Nature B.V. part of Springer Nature.
    Note
    12 month embargo; published 24 February 2021
    ISSN
    0921-8971
    EISSN
    1573-5176
    DOI
    10.1007/s10811-021-02409-z
    Version
    Final accepted manuscript
    Sponsors
    US Department of Energy
    ae974a485f413a2113503eed53cd6c53
    10.1007/s10811-021-02409-z
    Scopus Count
    Collections
    UA Faculty Publications

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