PCR-based gene targeting in Hanseniaspora uvarum

Author:

Badura Jennifer1,van Wyk Niël12ORCID,Zimmer Kerstin1,Pretorius Isak S2ORCID,von Wallbrunn Christian1,Wendland Jürgen1ORCID

Affiliation:

1. Department of Microbiology and Biochemistry, Hochschule Geisenheim University , Von-Lade-Strasse 1, 65366 Geisenheim , Germany

2. ARC Centre of Excellence in Synthetic Biology, Macquarie University , Sydney, NSW 2109 , Australia

Abstract

Abstract Lack of gene-function analyses tools limits studying the biology of Hanseniaspora uvarum, one of the most abundant yeasts on grapes and in must. We investigated a rapid PCR-based gene targeting approach for one-step gene replacement in this diploid yeast. To this end, we generated and validated two synthetic antibiotic resistance genes, pFA-hygXL and pFA-clnXL, providing resistance against hygromycin and nourseothricin, respectively, for use with H. uvarum. Addition of short flanking-homology regions of 56–80 bp to these selection markers via PCR was sufficient to promote gene targeting. We report here the deletion of the H. uvarum LEU2 and LYS2 genes with these marker genes via two rounds of consecutive transformations, each resulting in the generation of auxotrophic strains (leu2/leu2; lys2/lys2). The hereby constructed leucine auxotrophic leu2/leu2 strain was subsequently complemented in a targeted manner, thereby further validating this approach. PCR-based gene targeting in H. uvarum was less efficient than in Saccharomyces cerevisiae. However, this approach, combined with the availability of two marker genes, provides essential tools for directed gene manipulations in H. uvarum.

Funder

Australian Research Council

Publisher

Oxford University Press (OUP)

Subject

Applied Microbiology and Biotechnology,General Medicine,Microbiology

Reference46 articles.

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3. Synthesis of aroma compounds as a function of different nitrogen sources in fermentations using non-Saccharomyces wine yeasts;Badura;Microorganisms,2022

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