Literature DB >> 14663826

New modules for PCR-based gene targeting in Candida albicans: rapid and efficient gene targeting using 100 bp of flanking homology region.

Susanne Gola1, Ronny Martin, Andrea Walther, Alexander Dünkler, Jürgen Wendland.   

Abstract

The use of PCR-based techniques for directed gene alterations has become a standard tool in Saccharomyces cerevisiae. In our efforts to increase the speed of functional analysis of Candida albicans genes, we constructed a modular system of plasmid vectors and successfully applied PCR-amplified functional analysis (FA)-cassettes in the transformation of C. albicans. These cassettes facilitate: (a) gene disruptions; (b) tagging of 3'-ends of genes with green fluorescent protein (GFP); and (c) replacements of endogenous promoters to achieve regulated expression. The modules consists of a core of three selectable marker genes, CaURA3, CaHIS1 and CaARG4. Modules for C-terminal GFP-tagging were generated by adding GFP-sequences flanked at the 5'-end by a (Gly-Ala)3-linker and at the 3'-end by the S. cerevisiae URA3-terminator to these selection markers. Promoter exchange modules consist of the respective marker genes followed by the regulatable CaMAL2 or CaMET3 promoters at their 3'-ends. In order to ensure a reliably high rate of homologous gene targeting, the flanking homology regions required a size of 100 bp of gene-specific sequences, which were provided with the oligonucleotide primers. The use of shorter flanking homology regions produced unsatisfactory results with C. albicans strain BWP17. With these new modules only a minimal set of primers is required to achieve the functional analysis of C. albicans genes and, therefore, provides a basic tool to increase the number of functionally characterized C. albicans genes of this human pathogen in the near future. Copyright 2003 John Wiley & Sons, Ltd.

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Year:  2003        PMID: 14663826     DOI: 10.1002/yea.1044

Source DB:  PubMed          Journal:  Yeast        ISSN: 0749-503X            Impact factor:   3.239


  96 in total

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4.  Mms21: A Putative SUMO E3 Ligase in Candida albicans That Negatively Regulates Invasiveness and Filamentation, and Is Required for the Genotoxic and Cellular Stress Response.

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5.  Role for the SCFCDC4 ubiquitin ligase in Candida albicans morphogenesis.

Authors:  Avigail Atir-Lande; Tsvia Gildor; Daniel Kornitzer
Journal:  Mol Biol Cell       Date:  2005-04-06       Impact factor: 4.138

6.  Roles of calcineurin and Crz1 in antifungal susceptibility and virulence of Candida glabrata.

Authors:  Taiga Miyazaki; Shunsuke Yamauchi; Tatsuo Inamine; Yosuke Nagayoshi; Tomomi Saijo; Koichi Izumikawa; Masafumi Seki; Hiroshi Kakeya; Yoshihiro Yamamoto; Katsunori Yanagihara; Yoshitsugu Miyazaki; Shigeru Kohno
Journal:  Antimicrob Agents Chemother       Date:  2010-01-25       Impact factor: 5.191

7.  Ribosomal protein S6 phosphorylation is controlled by TOR and modulated by PKA in Candida albicans.

Authors:  Tahmeena Chowdhury; Julia R Köhler
Journal:  Mol Microbiol       Date:  2015-08-22       Impact factor: 3.501

8.  Promoter-dependent disruption of genes: simple, rapid, and specific PCR-based method with application to three different yeast.

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9.  Polarized hyphal growth in Candida albicans requires the Wiskott-Aldrich Syndrome protein homolog Wal1p.

Authors:  A Walther; J Wendland
Journal:  Eukaryot Cell       Date:  2004-04

10.  Carnitine-dependent transport of acetyl coenzyme A in Candida albicans is essential for growth on nonfermentable carbon sources and contributes to biofilm formation.

Authors:  Karin Strijbis; Carlo W T van Roermund; Wouter F Visser; Els C Mol; Janny van den Burg; Donna M MacCallum; Frank C Odds; Ekaterina Paramonova; Bastiaan P Krom; Ben Distel
Journal:  Eukaryot Cell       Date:  2008-02-15
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