Advantage of 16S rRNA amplicon sequencing in <i>Helicobacter pylori</i> diagnosis

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  • Boldbaatar Gantuya
    Department of Gastroenterology Mongolian National University of Medical Sciences Ulaanbaatar Mongolia
  • Hashem B. El Serag
    Department of Medicine, Gastroenterology and Hepatology Section Baylor College of Medicine Houston TX USA
  • Batsaikhan Saruuljavkhlan
    Department of Environmental and Preventive Medicine Oita University Faculty of Medicine Yufu Oita Japan
  • Dashdorj Azzaya
    Department of Environmental and Preventive Medicine Oita University Faculty of Medicine Yufu Oita Japan
  • Takashi Matsumoto
    Department of Environmental and Preventive Medicine Oita University Faculty of Medicine Yufu Oita Japan
  • Tomohisa Uchida
    Department of Molecular Pathology Oita University faculty of Medicine Yufu Oita Japan
  • Khasag Oyuntsetseg
    Department of Gastroenterology Mongolian National University of Medical Sciences Ulaanbaatar Mongolia
  • Nyamdorj Oyunbileg
    Department of Gastroenterology Mongolian National University of Medical Sciences Ulaanbaatar Mongolia
  • Duger Davaadorj
    Department of Gastroenterology Mongolian National University of Medical Sciences Ulaanbaatar Mongolia
  • Yoshio Yamaoka
    Department of Medicine, Gastroenterology and Hepatology Section Baylor College of Medicine Houston TX USA

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<jats:title>Abstract</jats:title><jats:sec><jats:title>Background</jats:title><jats:p>16S rRNA amplicon sequencing is an accurate method of detecting microbial infection without culture. It is unclear if sequencing has additional benefits over routine diagnostic methods for <jats:italic>Helicobacter</jats:italic> <jats:italic>pylori</jats:italic> testing.</jats:p></jats:sec><jats:sec><jats:title>Methods</jats:title><jats:p>We enrolled Mongolian volunteers with dyspepsia. Using routine diagnostic methods, positive <jats:italic>H</jats:italic>. <jats:italic>pylori</jats:italic> was defined as positive results on histology/immunohistochemistry, culture, rapid urease test, or serology; negative <jats:italic>H</jats:italic>. <jats:italic>pylori</jats:italic> was defined by negative results from all these tests. We performed 16S rRNA sequencing on gastric biopsy specimens and calculated cutoffs for operational taxonomic units (OTUs) and relative abundance (RA) to define positive results using ROC curves.</jats:p></jats:sec><jats:sec><jats:title>Results</jats:title><jats:p>We examined 161 individuals with a mean age of 43.6 years, and 64.6% were women. Using routine diagnostic methods, 122 (75.8%) participants were <jats:italic>H</jats:italic>. <jats:italic>pylori</jats:italic> positive, the sensitivity and specificity for 16S rRNA sequencing were 94.3% and 82.1% or 93.4% and 82.1% when cutoff values were set to 1113 (OTU number) or 4.4% RA, respectively (both <jats:italic>p</jats:italic> < .001). When combining the validated values, the concordance rate was high (91.1%); however, 16S rRNA sequencing had additional positive yield in 9 cases (5.6%) compared with routine diagnostic methods, and much greater additional positive yield compared to histopathology/IHC, culture, RUT, serology separately with 12 (7.4%), 37 (23.0%) and 43 (26.7%).</jats:p></jats:sec><jats:sec><jats:title>Conclusion</jats:title><jats:p>16S rRNA amplicon sequencing detects potentially important proportion of <jats:italic>H</jats:italic>. <jats:italic>pylori</jats:italic>‐positive cases that test negative with routine diagnostic methods. The quantitative number of <jats:italic>H</jats:italic>. <jats:italic>pylori</jats:italic> can help to understand how it can be changing by diseases and RA give opportunity to understand how <jats:italic>H</jats:italic>. <jats:italic>pylori</jats:italic> communicate with other microbiota.</jats:p></jats:sec>

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