In vivo genotoxicity testing strategies: Report from the 7th International workshop on genotoxicity testing (IWGT)

被引:33
|
作者
Kirkland, David [1 ]
Uno, Yoshifumi [2 ]
Luijten, Mirjam [3 ]
Beevers, Carol [4 ]
van Benthem, Jan [3 ]
Burlinson, Brian [5 ]
Dertinger, Stephen [6 ]
Douglas, George R. [7 ]
Hamada, Shuichi [8 ]
Horibata, Katsuyoshi [9 ]
Lovell, David P. [10 ]
Manjanatha, Mugimane [11 ]
Martus, Hans-Joerg [12 ]
Mei, Nan [11 ]
Morita, Takeshi [9 ]
Ohyama, Wakako [13 ]
Williams, Andrew [7 ]
机构
[1] Kirkland Consulting, POB 79, Tadcaster LS24 0AS, England
[2] Mitsubishi Tanabe Pharma Corp, 2-2-50 Kawagishi, Toda, Saitama 3358505, Japan
[3] Ctr Hlth Protect, Natl Inst Publ Hlth & Environm RVIM, Bilthoven, Netherlands
[4] Exponent Int Ltd, Hornbeam Pk, Harrogate HG2 8RE, England
[5] Envigo, Huntingdon PE28 4HS, Cambs, England
[6] Litron Labs, Rochester, NY USA
[7] Hlth Canada, Environm Hlth Sci Res Bur, Ottawa, ON K1A 0K9, Canada
[8] LSI Medience Corp, 14-1 Sunayama, Kamisu, Ibaraki 3140255, Japan
[9] Natl Inst Hlth Sci, 3-25-26 Tonomachi, Kawasaki, Kanagawa 2109501, Japan
[10] Univ London, St Georges Med Sch, London SW17 0RE, England
[11] US FDA, Natl Ctr Toxicol Res, Jefferson, AR 72079 USA
[12] Novartis Inst Biomed Res, Basel, Switzerland
[13] Yakult Honsha Co Ltd, 5-11 Izumi, Kunitachi, Tokyo 1868650, Japan
关键词
Genotoxicity in vivo; Transgenic rodent mutation; In vivo comet assay; In vivo micronucleus; Pig-a assay; Risk assessment; A GENE MUTATION; MOUSE BONE-MARROW; CD48-DEFICIENT T-LYMPHOCYTES; UPPER GASTROINTESTINAL-TRACT; GEL-ELECTROPHORESIS ASSAY; RODENT MICRONUCLEUS ASSAY; CELL-SPECIFIC METHYLATION; COLLABORATIVE STUDY-GROUP; ETHYL-N-NITROSOUREA; RED-BLOOD-CELLS;
D O I
10.1016/j.mrgentox.2019.03.008
中图分类号
Q81 [生物工程学(生物技术)]; Q93 [微生物学];
学科分类号
071005 ; 0836 ; 090102 ; 100705 ;
摘要
The working group reached complete or majority agreement on many issues. Results from TGR and in vivo comet assays for 91 chemicals showed they have similar ability to detect in vivo genotoxicity per se with bacterial mutagens and Ames-positive carcinogens. TGR and comet assay results were not significantly different when compared with IARC Group 1, 2 A, and unclassified carcinogens. There were significantly more comet assay positive responses for Group 2B chemicals, and for IARC classified and unclassified carcinogens combined, which may be expected since mutation is a subset of genotoxicity. A liver comet assay combined with the bone marrow/blood micronucleus (MNviv) test would detect in vivo genotoxins that do not exhibit tissue-specific or site-of-contact effects, and is appropriate for routine in vivo genotoxicity testing. Generally for orally administered substances, a comet assay at only one site-of-contact GI tract tissue (stomach or duodenum/jejunum) is required. In MNviv tests, evidence of target tissue exposure can be obtained in a number of different ways, as recommended by ICH S2(R1) and EFSA (Hardy et al., 2017). Except for special cases the i.p. route is inappropriate for in vivo testing; for risk evaluations more weight should be given to data from a physiologically relevant administration route. The liver MN test is sufficiently validated for the development of an OECD guideline. However, the impact of dosing animals > 6 weeks of age needs to be evaluated. The GI tract MN test shows promise but needs more validation for an OECD guideline. The Pig-a assay detects systemically available mutagens and is a valuable follow-up to in vitro positive results. A new freeze-thaw protocol provides more flexibility. Mutant reticulocyte and erythrocyte frequencies should both be determined. Preliminary data are available for the Pig a assay in male rat germ cells which require validation including germ cell DNA mutation orgin.
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页数:24
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