A comprehensive fungi-specific 18S rRNA gene sequence primer toolkit suited for diverse research issues and sequencing platforms.

Banos, Stefanos; Lentendu, Guillaume; Kopf, Anna; Wubet, Tesfaye; Glöckner, Frank Oliver; Reich, Marlis

Banos, Stefanos; Lentendu, Guillaume; Kopf, Anna; Wubet, Tesfaye; Glöckner, Frank Oliver; Reich, Marlis.

Afiliação

Banos S; Molecular Ecology, Institute of Ecology, FB02, University of Bremen, Leobener Str. 2, 28359, Bremen, Germany.
Lentendu G; Department of Soil Ecology, Helmholtz Centre for Environmental Research GmbH - UFZ, Halle-Saale, Germany.
Kopf A; Department of Ecology, University of Kaiserslautern, Kaiserslautern, Germany.
Wubet T; Microbial Genomics and Bioinformatics Research Group, Max Planck Institute for Marine Microbiology, Bremen, Germany.
Glöckner FO; Department of Soil Ecology, Helmholtz Centre for Environmental Research GmbH - UFZ, Halle-Saale, Germany.
Reich M; Present address: Department of Community Ecology, Helmholtz Centre for Environmental Research GmbH - UFZ, Halle-Saale, Germany.

BMC Microbiol ; 18(1): 190, 2018 11 20.

Article em En | MEDLINE | ID: mdl-30458701

ABSTRACT

ABSTRACT

BACKGROUND:

Several fungi-specific primers target the 18S rRNA gene sequence, one of the prominent markers for fungal classification. The design of most primers goes back to the last decades. Since then, the number of sequences in public databases increased leading to the discovery of new fungal groups and changes in fungal taxonomy. However, no reevaluation of primers was carried out and relevant information on most primers is missing. With this study, we aimed to develop an 18S rRNA gene sequence primer toolkit allowing an easy selection of the best primer pair appropriate for different sequencing platforms, research aims (biodiversity assessment versus isolate classification) and target groups.

RESULTS:

We performed an intensive literature research, reshuffled existing primers into new pairs, designed new Illumina-primers, and annealing blocking oligonucleotides. A final number of 439 primer pairs were subjected to in silico PCRs. Best primer pairs were selected and experimentally tested. The most promising primer pair with a small amplicon size, nu-SSU-1333-5'/nu-SSU-1647-3' (FF390/FR-1), was successful in describing fungal communities by Illumina sequencing. Results were confirmed by a simultaneous metagenomics and eukaryote-specific primer approach. Co-amplification occurred in all sample types but was effectively reduced by blocking oligonucleotides.

CONCLUSIONS:

The compiled data revealed the presence of an enormous diversity of fungal 18S rRNA gene primer pairs in terms of fungal coverage, phylum spectrum and co-amplification. Therefore, the primer pair has to be carefully selected to fulfill the requirements of the individual research projects. The presented primer toolkit offers comprehensive lists of 164 primers, 439 primer combinations, 4 blocking oligonucleotides, and top primer pairs holding all relevant information including primer's characteristics and performance to facilitate primer pair selection.

Assuntos

Primers do DNA/genética; DNA Fúngico/genética; RNA Ribossômico 18S/genética; Biodiversidade; Fungos/classificação; Fungos/genética; Fungos/isolamento & purificação; Sequenciamento de Nucleotídeos em Larga Escala; Reação em Cadeia da Polimerase; Especificidade da Espécie

Palavras-chave

18S rRNA gene sequence (SSU) primer; Annealing blocking oligonucleotides; Co-amplification; Community survey; FF390; FR-1; Fungal biodiversity; Fungi; Real-time Q-PCR; Taxonomic classification

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Texto completo: 1 Coleções: 01-internacional Base de dados: MEDLINE Assunto principal: DNA Fúngico / RNA Ribossômico 18S / Primers do DNA Idioma: En Revista: BMC Microbiol Ano de publicação: 2018 Tipo de documento: Article

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