Pro‐inflammatory activity of Cutibacterium acnes phylotype IA1 and extracellular vesicles: An in vitro study

Author:

Cheung Caroline T.1ORCID,Lancien Ugo2,Corvec Stéphane13,Mengeaud Valérie4,Mias Céline5,Véziers Joëlle6,Khammari Amir17,Dréno Brigitte1ORCID

Affiliation:

1. Nantes University, INSERM, CNRS, Immunology and New Concepts in ImmunoTherapy (INCIT) Nantes France

2. Nantes University, CHU Nantes Chirurgie Plastique, Reconstructrice et Esthétique et Centre de traitement des Brûlés, Hôtel‐Dieu Nantes France

3. CHU Nantes Bacteriology Department Nantes University Nantes France

4. Medical Direction, Laboratoires Dermatologiques Ducray, Les Cauquillous Lavaur France

5. Pierre Fabre Dermo‐Cosmétique et Personal Care Toulouse France

6. Nantes University, Oniris, CHU Nantes, INSERM, Regenerative Medicine and Skeleton, RMeS Nantes France

7. Department of Dermatology Nantes University, CHU Nantes, INSERM Nantes France

Abstract

AbstractAcne is a chronic inflammatory skin condition that involves Cutibacterium acnes (C. acnes), which is classified into six main phylotypes (IA1, IA2, IB, IC, II and III). Acne development is associated with loss of C. acnes phylotype diversity, characterised by overgrowth of phylotype IA1 relative to other phylotypes. It was also shown that purified extracellular vesicles (EVs) secreted by C. acnes can induce an acne‐like inflammatory response in skin models. We aimed to determine if the inflammatory profile of EVs secreted by C. acnes phylotype IA1 from an inflammatory acne lesion was different from C. acnes phylotype IA1 from normal skin, thus playing a direct role in the severity of inflammation. EVs were produced in vitro after culture of two clinical strains of C. acnes phylotype IA1, T5 from normal human skin and A47 from an inflammatory acne lesion, and then incubated with either human immortalised keratinocytes, HaCaT cells, or skin explants obtained from abdominoplasty. Subsequently, quantitative PCR (qPCR) was performed for human β‐defensin 2 (hBD2), cathelicidin (LL‐37), interleukin (IL)‐1β, IL‐6, IL‐8, IL‐17α and IL‐36γ, and ELISA for IL‐6, IL‐8 and IL‐17α. We found that EVs produced in vitro by C. acnes derived from inflammatory acne lesions significantly increased the pro‐inflammatory cytokines and anti‐microbial peptides at both transcriptional and protein levels compared with EVs derived from normal human skin. We show for the first time that C. acnes EVs from inflammatory acne play a crucial role in acne‐associated inflammation in vitro and that C. acnes phylotype IA1 collected from inflammatory acne lesion and normal skin produce different EVs and inflammatory profiles in vitro.

Publisher

Wiley

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