Comparison of two primer-probe sets of Fusobacterium nucleatum using droplet digital polymerase chain reaction for the detection of colorectal neoplasia from faecal samples

Author:

Yamaoka Yuko1,Sasai Mai23,Suehiro Yutaka3ORCID,Hashimoto Shinichi1,Goto Atsushi1,Yamamoto Naoki1,Suzuki Nobuaki4,Higaki Shingo5,Fujii Ikuei6,Suzuki Chieko6ORCID,Matsumoto Toshihiko12,Hoshida Tomomi2,Koga Michiko7,Tsutsumi Takeya7,Lim Lay A8,Matsubara Yasuo8,Tomochika Shinobu4,Yoshida Shin4,Hazama Shoichi9,Yotsuyanagi Hiroshi7,Nagano Hiroaki4,Sakaida Isao5,Takami Taro1,Yamasaki Takahiro23

Affiliation:

1. Department of Gastroenterology and Hepatology, Yamaguchi University Graduate School of Medicine, Ube, Japan

2. Division of Laboratory, Yamaguchi University Hospital, Ube, Japan

3. Department of Oncology and Laboratory Medicine, Yamaguchi University Graduate School of Medicine, Ube, Japan

4. Department of Digestive Surgery and Surgical Oncology, Yamaguchi University Graduate School of Medicine, Ube, Japan

5. Department of Gastroenterology, St. Hill Hospital, Ube, Japan

6. Ajisu Kyoritsu Hospital, Yamaguchi, Japan

7. Division of Infectious Diseases, The Advanced Clinical Research Centre, The Institute of Medical Science, The University of Tokyo, Tokyo, Japan

8. Department of General Medicine, IMSUT Hospital, The Institute of Medical Science, The University of Tokyo, Tokyo, Japan

9. Department of Translational Research and Developmental Therapeutics Against Cancer, Yamaguchi University Graduate School of Medicine, Ube, Japan

Abstract

Background: Although faecal DNA testing of Fusobacterium nucleatum ( Fn) is expected to be useful for colorectal neoplasia detection, there is no standardized quantification method of Fn. We performed this study to establish a possible standardized method. Methods: In this study, 322 participants including 71 subjects without colorectal neoplasia (control group), 31 patients with non-advanced colorectal adenoma, 93 patients with advanced colorectal adenoma, and 127 patients with colorectal cancer were enrolled. Faecal Fn were quantified by droplet digital PCR (ddPCR) using two PCR primer-probe sets reported previously that are tentatively named Fn1 and Fn2. Fn1 has been used in ddPCR by us and Fn2 has been widely used in quantitative real-time PCR. Results: The Fn copy number using Fn1 was five times higher than that using Fn2, with a linear relationship shown between them. Receiver operating characteristic curve analysis showed the area under the curve (AUC) to be almost the same between Fn1 and Fn2 in discriminating between the control group and the colorectal cancer group (AUC = 0.81 and 0.81, respectively), and between the control/non-advanced colorectal adenoma group and the advanced colorectal adenoma/colorectal cancer group (AUC = 0.74 and 0.74, respectively). Conclusions: As the diagnostic performance was quite similar between Fn1 and Fn2, ddPCR-based Fn testing using Fn1 and Fn2 could be a possible standardized method for a colorectal neoplasia screening test, considering that Fn levels quantified by Fn1 are about five times higher than those by Fn2.

Funder

Japan Society for the Promotion of Science

Publisher

SAGE Publications

Subject

Clinical Biochemistry,General Medicine

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