In vitro assessment of genotoxicity in living cells: the

In vitro assessment of genotoxicity in living cells:

the pluripotent stem cell micronucleus assay (PMNvit)

CF Lerche, BN Hölzel, P Stahlschmidt-Allner, B Allner

Overview

SETAC GLB Annual Meeting 2017 Dr. Cristiano F. Lerche

Genotoxicity testing

Prokaryotes (S. typhimurium, E. coli)

MLA (TK+/-), HPRT

Comet assay, Chromosome aberrationMicronucleus assay

Eukaryotes / Vertebrates(in vivo / ex-vivo, rodent cells)

SOS chromotest(umu assay)

Direct DNA damage(e.g. mutations)

Direct DNA damageDouble strand breakage

Mitotic apparatus failure

https://sciencealert.com

(mutations)

(epigenetic)

Micronucleus formation

Ferench, M., 2007. Nat. Prot.

MN formation:

Chromosome breakage (clastogens)

Chromosome loss (aneugens)

Karryorhexis (fragmentation of nuclei):

Apoptosis (preceded by pyknosis)

Necrosis

Micronucleus assay

In vivo (ex-vivo): OECD TG 474 (mammalian erythrocytes)

In vitro: OECD TG 487 (human peripheral blood lymphocytes, rodent immortalized cell lines e.g. CHO, V79)

Exposure to test compounds

Transfer of cells to microscope slides

Fixation and nuclear staining(e.g. Giemsa, acridine orange)

El-Zain et al. 2008. Cancer Epidemiol. Biom. Prev.

Microscopic scoring of MN-frequency

Alternatively: Flow cytometry methods(e.g. Torous et al. 2005, De Boeck et al. 2005)

Micronucleus Frequencies and Carcinogenesis

Dose-response, threshold dose and LOAEL

El-Zain et al. 2008. Cancer Epidemiol. Biom. Prev.,17(5): 1111-1119.

Bonassi et al. 2007. Carcinogenesis, 28 (3): 625–631.

Micronuclei, nucleoplasmic bridges, and nuclear

buds in lymphocytes as predictors of cancer risk

Chromotripsise.g. Stephens et al. 2011.

Cell, 144(1): 27 – 40.

Micronucleie.g. Zhang et al. 2015.Nature 522: 179–184.

Threshold

KCB-GFP = DSM ACC3285 Budapest treaty

26°C growth temperature / no CO2

Cell line

10 µm

Epigenetic defects

The pluripotent stem cell micronucleus assay - PMNvit

Automatic shooting of pictures and cell counting

Evaluation of MN frequencies(optionally also of FN frequencies)

Pre-cultivated cells stored at 4° C

Replace medium and allow for recovery(60% monolayer confluence)

Exposure in culture medium

Passaging for downstream analysis

Range Finding

Normal celllayer

Cytotoxiceffect

Genotoxicity testing

Concentration range

Cell count

Concretecriteria

MN frequency evaluation

Cell counting

Fluorescence intensity(e.g. pyknosis)

Manual evaluation:

Micronuclei

Fragmentednuclei

Colchicine (aneugen)

C22H25NO6

Significant (p<0.0001)

4-Nitroquinoline 1-oxide (clastogen)

C9H6N2O3

Significant (p<0.0001)

Cytokinesis blocker (Cytochalasin B)

C29H37NO5

Significant (p=0.0012)

Cyclophosphamide (metabolic activation)

C7H15Cl2N2O2P

Significant (p=0.0046)

Ethyl methanesulfonate & diethylstilbestrol

Ethyl methanesulfonate (EMS) Diethylstilbestrol (DES)

Not significant (p=0.11) Significant (p=0.0086)

PMNvit pre-validation

Aneugens (e.g. colchicine)

Natural clastogens (e.g. 4-NQO)

Clastogens after metabolic activation (e.g. Cyclophosphamide)

Cytokinesis blocker

Further applications I

Background research

Further applications II

Downstream analysis

Fluorescence intensity

Elongated / deformed nuclei

Proliferation rate

Perspectives

Inter-laboratory comparison - RWTH Aachen University(metabolic activation)

Validation and certification

Automatic assessment of MN(software)

Round robin tests

Acknowledgements

J Hescheler, K Pfannkuche, D Derichsweiler ZIM ZF4066801MD5

In vitro assessment of genotoxicity in living cells: the

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