The suitability of micronuclei as markers of relative biological effect

Charlotte J Heaven; Hannah C Wanstall; Nicholas T Henthorn; John-William Warmenhoven; Samuel P Ingram; Amy L Chadwick; Elham Santina; Jamie Honeychurch; Christine K Schmidt; Karen J Kirkby; Norman F Kirkby; Neil G Burnet; Michael J Merchant

doi:10.1093/mutage/geac001

The suitability of micronuclei as markers of relative biological effect

Mutagenesis. 2022 Apr 2;37(1):3-12. doi: 10.1093/mutage/geac001.

Authors

Charlotte J Heaven^{1

2}, Hannah C Wanstall^{2

3}, Nicholas T Henthorn^{1

2}, John-William Warmenhoven^{1

2}, Samuel P Ingram^{1

4}, Amy L Chadwick¹, Elham Santina¹, Jamie Honeychurch¹, Christine K Schmidt¹, Karen J Kirkby^{1

2}, Norman F Kirkby^{1

2}, Neil G Burnet², Michael J Merchant^{1

2}

Affiliations

¹ Division of Cancer Sciences, Faculty of Biology, Medicine and Health, School of Medical Sciences, The University of Manchester, Oxford Road, M13 9PL Manchester, United Kingdom.
² Manchester Academic Health Science Centre, The Christie NHS Foundation Trust, Wilmslow Road, M20 4BX Manchester, United Kingdom.
³ Department of Physics and Astronomy, Faculty of Science and Engineering, The University of Manchester, Oxford Road, M13 9PL Manchester, United Kingdom.
⁴ Christie Medical Physics and Engineering, The Christie NHS Foundation Trust, Wilmslow Road, M20 4BX Manchester, United Kingdom.

Abstract

Micronucleus (MN) formation is routinely used as a biodosimeter for radiation exposures and has historically been used as a measure of DNA damage in cells. Strongly correlating with dose, MN are also suggested to indicate radiation quality, differentiating between particle and photon irradiation. The "gold standard" for measuring MN formation is Fenech's cytokinesis-block micronucleus (CBMN) cytome assay, which uses the cytokinesis blocking agent cytochalasin-B. Here, we present a comprehensive analysis of the literature investigating MN induction trends in vitro, collating 193 publications, with 2476 data points. Data were collected from original studies that used the CBMN assay to quantify MN in response to ionizing radiation in vitro. Overall, the meta-analysis showed that individual studies mostly have a linear increase of MN with dose [85% of MN per cell (MNPC) datasets and 89% of percentage containing MN (PCMN) datasets had an R2 greater than 0.90]. However, there is high variation between studies, resulting in a low R2 when data are combined (0.47 for MNPC datasets and 0.60 for PCMN datasets). Particle type, species, cell type, and cytochalasin-B concentration were suggested to influence MN frequency. However, variation in the data meant that the effects could not be strongly correlated with the experimental parameters investigated. There is less variation between studies when comparing the PCMN rather than the number of MNPC. Deviation from CBMN protocol specified timings did not have a large effect on MN induction. However, further analysis showed less variation between studies following Fenech's protocol closely, which provided more reliable results. By limiting the cell type and species as well as only selecting studies following the Fenech protocol, R2 was increased to 0.64 for both measures. We therefore determine that due to variation between studies, MN are currently a poor predictor of radiation-induced DNA damage and make recommendations for futures studies assessing MN to improve consistency between datasets.

Keywords: DNA damage; cytochalasin-B; micronuclei; radiotherapy.

Publication types

Meta-Analysis
Research Support, Non-U.S. Gov't

MeSH terms

Cytokinesis*
DNA Damage
Lymphocytes*
Micronucleus Tests / methods
Radiation, Ionizing

Abstract

Publication types

MeSH terms

Grants and funding