Extension of bacterial rDNA sequencing for simultaneous methylation detection and its application in microflora analysis

Motoi Nishimura; Tomoaki Tanaka; Syota Murata; Akiko Miyabe; Takayuki Ishige; Kenji Kawasaki; Masataka Yokoyama; Naoko Hashimoto; Kazuyuki Yamagata; Hidekazu Nagano; Satomi Tojo-Nishimura; Kazuyuki Matsushita

doi:10.1038/s41598-023-28706-w

Scientific Reports (Apr 2023)

Extension of bacterial rDNA sequencing for simultaneous methylation detection and its application in microflora analysis

Motoi Nishimura,
Tomoaki Tanaka,
Syota Murata,
Akiko Miyabe,
Takayuki Ishige,
Kenji Kawasaki,
Masataka Yokoyama,
Naoko Hashimoto,
Kazuyuki Yamagata,
Hidekazu Nagano,
Satomi Tojo-Nishimura,
Kazuyuki Matsushita

Affiliations

Motoi Nishimura: Division of Laboratory Medicine, Clinical Genetics and Proteomics, Chiba University Hospital
Tomoaki Tanaka: Department of Molecular Diagnosis, Graduate School of Medicine, Chiba University
Syota Murata: Division of Laboratory Medicine, Clinical Genetics and Proteomics, Chiba University Hospital
Akiko Miyabe: Division of Laboratory Medicine, Clinical Genetics and Proteomics, Chiba University Hospital
Takayuki Ishige: Division of Laboratory Medicine, Clinical Genetics and Proteomics, Chiba University Hospital
Kenji Kawasaki: Division of Laboratory Medicine, Clinical Genetics and Proteomics, Chiba University Hospital
Masataka Yokoyama: Department of Molecular Diagnosis, Graduate School of Medicine, Chiba University
Naoko Hashimoto: Department of Molecular Diagnosis, Graduate School of Medicine, Chiba University
Kazuyuki Yamagata: Department of Molecular Diagnosis, Graduate School of Medicine, Chiba University
Hidekazu Nagano: Department of Molecular Diagnosis, Graduate School of Medicine, Chiba University
Satomi Tojo-Nishimura: Department of Molecular Diagnosis, Graduate School of Medicine, Chiba University
Kazuyuki Matsushita: Division of Laboratory Medicine, Clinical Genetics and Proteomics, Chiba University Hospital

DOI: https://doi.org/10.1038/s41598-023-28706-w
Journal volume & issue: Vol. 13, no. 1
pp. 1 – 12

Abstract

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Abstract Although polymerase chain reaction (PCR) amplification and sequencing of the bacterial 16S rDNA region has numerous scientific applications, it does not provide DNA methylation information. Herein, we propose a simple extension for bisulfite sequencing to investigate 5-methylcytosine residues in the bacterial 16S rDNA region from clinical isolates or flora. Multiple displacement amplification without DNA denaturation was used to preferentially pre-amplify single-stranded bacterial DNA after bisulfite conversion. Following the pre-amplification, the 16S rDNA region was analyzed using nested bisulfite PCR and sequencing, enabling the simultaneous identification of DNA methylation status and sequence data. We used this approach (termed sm16S rDNA PCR/sequencing) to identify novel methylation sites and a methyltransferase (M. MmnI) in Morganella morganii and different methylation motifs among Enterococcus faecalis strains from small volumes of clinical specimens. Further, our analysis suggested that M. MmnI may be correlated to erythromycin resistance. Thus, sm16S rDNA PCR/sequencing is a useful extension method for analyzing the DNA methylation of 16S rDNA regions in a microflora, providing additional information not provided by conventional PCR. Given the relationship between DNA methylation status and drug resistance in bacteria, we believe this technique can be effectively applied in clinical sample testing.

Published in Scientific Reports

ISSN: 2045-2322 (Online)
Publisher: Nature Portfolio
Country of publisher: United Kingdom
LCC subjects: Medicine; Science
Website: https://www.nature.com/srep/

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