An experimental aerosol air-agar interface mouse lymphoma assay methodology

D Thorne; M Hollings; J Kilford; J Clements; R Payne; M Ballantyne; A Dalrymple; D Dillon; C Meredith; M Gaҫa

doi:10.1016/j.mrgentox.2020.503230

An experimental aerosol air-agar interface mouse lymphoma assay methodology

Mutat Res Genet Toxicol Environ Mutagen. 2020 Aug-Sep:856-857:503230. doi: 10.1016/j.mrgentox.2020.503230. Epub 2020 Jul 13.

Authors

D Thorne¹, M Hollings², J Kilford², J Clements², R Payne², M Ballantyne², A Dalrymple³, D Dillon³, C Meredith³, M Gaҫa³

Affiliations

¹ British American Tobacco, R&D, Southampton, Hampshire, SO15 8TL, UK. Electronic address: David_Thorne@bat.com.
² Covance Laboratories Ltd., Otely Road, Harrogate, HG1 PY, UK.
³ British American Tobacco, R&D, Southampton, Hampshire, SO15 8TL, UK.

PMID: 32928375
DOI: 10.1016/j.mrgentox.2020.503230

Abstract

This work investigates a completely novel and experimental concept of exposing L5178Y cells at the air-agar-interface to mainstream cigarette smoke aerosol (Kentucky reference 3R4F). This study highlights the associated challenges of combining a suspension cell line alongside an in vitro aerosol exposure system. To achieve a monolayer, cells were 'seeded' in a concentrated cell super-mix suspension onto an RPMI/agar-matrix -base. The resulting cell suspension media was adsorbed into the agar base leaving the L5178Y cells lightly suspended on the agar surface, approximating a monolayer. Cells were deemed supportable on the agar-matrix, viable and recoverable. Using Vitrocell VC 10 exposure system and the Ames 4 exposure module, L5178Y cells were successfully exposed to a dynamic cigarette smoke aerosol, recovered and assessed for mutant frequencies, using standard assay procedures. Method development included assessment of flowing air conditions, plating efficiency and recovery of L5178Y cells from the agar-matrix surface. Positive controls MMS and B[a]P were successfully incorporated into the agar-matrix and metabolic activation was achieved by S-9 incorporation into the same agar-base-matrix. B[a]P demonstrated metabolic activation and positive response, suggesting a clear cellular interaction with the agar-matrix. Whole smoke exposed cells in the presence of metabolic activation showed a clear dose response and increasing mutant frequencies, well in excess of the controls (air and incubator) and the global evaluation factor following a 2 or 3 day expression period. This experimental concept demonstrates that L5178Y cells can be exposed to cigarette smoke aerosol, using a completely novel and a previously untested approach. Although this work successfully demonstrates the approach is viable and cells can be plated and maintained on an agar-matrix, more optimisation and robustness assessment is required before it can be considered fully adapted and used alongside other whole aerosol methodologies for the assessment of cigarette smoke and other inhaled aerosols.

Keywords: 3R4F cigarette; Aerosol; Air–agar interface; In vitro; MLA; Vitrocell® VC10® exposure system.

Publication types

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

MeSH terms

Aerosols / pharmacology
Aerosols / toxicity
Agar / chemistry
Air
Animals
Cell Line / drug effects
Dose-Response Relationship, Drug
Electronic Nicotine Delivery Systems
Humans
Lymphoma / chemically induced
Lymphoma / pathology*
Mice
Mutagenicity Tests*
Mutagens / pharmacology
Mutagens / toxicity*
Smoke / adverse effects*

Substances

Aerosols
Mutagens
Smoke
Agar