Evaluation of the novel liver micronucleus assay using formalin-fixed tissues

Shuichi Hamada; Miyuki Shigano; Satoru Kawakami; Maya Ueda; Hajime Sui; Katsuya Yamada; Soichiro Hagio; Ayaka Momonami; Akihisa Maeda; Yukari Terashima; Wakako Ohyama; Takeshi Morita; Makoto Hayashi

doi:10.1186/s41021-019-0128-5

Evaluation of the novel liver micronucleus assay using formalin-fixed tissues

Genes Environ. 2019 May 9:41:13. doi: 10.1186/s41021-019-0128-5. eCollection 2019.

Authors

Affiliations

¹ Safety Assessment Department, Nonclinical Research Center, Drug Development Service Segment, LSI Medience Corporation, 14-1, Sunayama, Kamisu-shi, Ibaraki, 314-0255 Japan.
² 2Asahi Kasei Pharma Corporation, 632-1 Mifuku, Izunokuni-shi, Shizuoka, 410-2321 Japan.
³ BioSafety Research Center Inc., 582-2 Shioshinden, Iwata-shi, Shizuoka, 437-1213 Japan.
⁴ 4Food and Drug Safety Center, 729-5 Ochiai, Hadano-shi, Kanagawa 257-8523 Japan.
⁵ 5Mitsubishi Tanabe Pharma Corporation, 2-2-50 Kawagishi, Toda-shi, Saitama, 335-8505 Japan.
⁶ Nissan Chemical Corporation, 1470 Shiraoka, Shiraoka-shi, Saitama, 349-0294 Japan.
⁷ Suntory MONOZUKURI Expert Ltd., 8-1-1 Seikadai, Seika-cho, Soraku-gun, Kyoto, 619-0284 Japan.
⁸ 8Toray Industries Inc., 6-10-1 Tebiro, Kamakura-shi, Kanagawa 248-8555 Japan.
⁹ 9Kissei Pharmaceutical Co., Ltd., 2320-1 Maki, Hotaka, Azumino-shi, Nagano, 399-8305 Japan.
¹⁰ 10Yakult Honsha Co., Ltd., 5-11 Izumi, Kunitachi-shi, Tokyo, 186-8650 Japan.
¹¹ 11National Institute of Health Sciences, 3-25-26 Tonomachi, Kawasaki-shi, Kanagawa 210-9501 Japan.
¹² makoto international consulting, 4-23-3-1 Kamiimaizumi, Ebina-shi, Kanagawa 243-0431 Japan.

Abstract

Background: The repeated-dose liver micronucleus (RDLMN) assay is an effective and important in vivo test for detecting genotoxic compounds, particularly for those that require metabolic activation to show genotoxicity. In a collaborative study by the Collaborative Study Group for the Micronucleus Test (CSGMT)/The Japanese Environmental Mutagen Society (JEMS) - Mammalian Mutagenicity Study Group (MMS), micronucleus induction of 22 chemicals with the RDLMN assay employing the collagenase digestion method was examined and reported on. Recently, we have developed a method which enables retrospective evaluation of micronucleus induction in formalin-fixed liver tissues (the formalin-fixed method) obtained in general toxicity studies completed in the past. Using this method, we were able to easily evaluate clastogenic potential of chemicals from the formalin-fixed tissues obtained in the general toxicity studies.In this study, to evaluate the usefulness of the formalin-fixed method, we have conducted a liver micronucleus assay using the formalin-fixed liver samples obtained from the above collaborative study (18 of 22 test chemicals) and carried out a comparison with the results obtained by the collagenase digestion method.

Results: Comparison of the collagenase digestion and formalin-fixed methods was conducted using the results of the micronucleus assays with a total of 18 test chemicals which included 12 genotoxic hepatocarcinogens (Group A), 4 genotoxic carcinogens but not liver targeted (Group B), and 2 nongenotoxic hepatocarcinogens (Group C). The formalin-fixed method obtained the similar results as the collagenase digestion method in 10 out of the 12 chemicals of Group A, and all chemicals of Group B and Group C. Although the results were statistically contradictive due to different levels of concurrent negative control, the 2 other chemicals of Group A showed comparable responses between the two methods.

Conclusion: The present study shows that the formalin-fixed method is capable of detecting liver carcinogens with sensitivity equal to or higher than that of the collagenase digestion method. We recommend use of the formalin-fixed method because of its capability of enabling retrospective evaluation of micronucleus induction in the formalin-fixed liver tissues obtained in general toxicity studies completed in the past.

Keywords: Collagenase; Formalin-fixed tissue; Hepatocyte; Liver; Micronucleus assay.