Assessing testicular germ cell DNA damage in the comet assay; introduction of a proof‐of‐concept

Author:

Dirven Yvette12,Eide Dag Markus12,Henriksson Erika Witasp34,Hjorth Rune5,Sharma Anoop Kumar6,Graupner Anne12,Brunborg Gunnar12,Ballangby Jarle12,Boisen Anne Mette Zenner6,Swedmark Stellan4,Gützkow Kristine Bjerve12,Olsen Ann‐Karin12

Affiliation:

1. Norwegian Institute of Public Health Division of Climate and Environmental Health Oslo Norway

2. Centre for Environmental Radioactivity (CERAD, Centre of Excellence of the Norwegian Research Council) Oslo Norway

3. Swedish Chemicals Agency, Department of Development of Legislation and Other Instruments Unit of Proposals for Classification and Restriction Sundbyberg Sweden

4. Swedish Chemicals Agency, Department of Development of Legislation and Other Instruments Unit of Evaluation of Substances Sundbyberg Sweden

5. The Danish Environmental Protection Agency Odense Denmark

6. Technical University of Denmark National Food Institute Lyngby Denmark

Abstract

AbstractThe in vivo comet assay is widely used to measure genotoxicity; however, the current OECD test guideline (TG 489) does not recommend using the assay to assess testicular germ cells, due to the presence of testicular somatic cells. An adapted approach to specifically assess testicular germ cells within the comet assay is certainly warranted, considering regulatory needs for germ cell‐specific genotoxicity data in relation to the increasing global production of and exposure to potentially hazardous chemicals. Here, we provide a proof‐of‐concept to selectively analyze round spermatids and primary spermatocytes, distinguishing them from other cells of the testicle. Utilizing the comet assay recordings of DNA content (total fluorescence intensity) and DNA damage (% tail intensity) of individual comets, we developed a framework to distinguish testicular cell populations based on differences in DNA content/ploidy and appearance. Haploid round spermatid comets are identified through (1) visual inspection of DNA content distributions, (2) setting DNA content thresholds, and (3) modeling DNA content distributions using a normal mixture distribution function. We also describe an approach to distinguish primary spermatocytes during comet scoring, based on their high DNA content and large physical size. Our concept allows both somatic and germ cells to be analyzed in the same animal, adding a versatile, sensitive, rapid, and resource‐efficient assay to the limited genotoxicity assessment toolbox for germ cells. An adaptation of TG 489 facilitates accumulation of valuable information regarding distribution of substances to germ cells and their potential for inducing germ cell gene mutations and structural chromosomal aberrations.

Funder

Nordisk Ministerråd

Publisher

Wiley

Subject

Health, Toxicology and Mutagenesis,Genetics (clinical),Epidemiology

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