Full‐spectrum cannabidiol reduces UVB damage through the inhibition of TGF‐β1 and the NLRP3 inflammasome

Author:

Urrutia‐Ortega I. M.12ORCID,Valencia I.2ORCID,Ispanixtlahuatl‐Meraz O.1,Benítez‐Flores J. C.3,Espinosa‐González A. M.2,Estrella‐Parra E. A.2,Flores‐Ortiz C. M.45,Chirino Y. I.1,Avila‐Acevedo J. G.2ORCID

Affiliation:

1. Laboratorio de Carcinogénesis y Toxicología, Unidad de Investigación en Biomedicina, Facultad de Estudios Superiores Iztacala Universidad Nacional Autónoma de México Tlalnepantla de Baz Estado de México Mexico

2. Laboratorio de Fitoquímica, Unidad de Biotecnología y Prototipos, Facultad de Estudios Superiores Iztacala Universidad Nacional Autónoma de México Tlalnepantla de Baz Estado de México Mexico

3. Laboratorio de Histología, Unidad de Morfología y Función, Facultad de Estudios Superiores Iztacala Universidad Nacional Autónoma de México Tlalnepantla de Baz Estado de México Mexico

4. Laboratorio de Fisiología Vegetal, Facultad de Estudios Superiores Iztacala Universidad Nacional Autónoma de México Tlalnepantla de Baz Estado de México Mexico

5. Laboratorio Nacional en Salud, Facultad de Estudios Superiores Iztacala Universidad Nacional Autónoma de México Tlalnepantla de Baz Estado de México Mexico

Abstract

AbstractThe thermodynamic characteristics, antioxidant potential, and photoprotective benefits of full‐spectrum cannabidiol (FS‐CBD) against UVB‐induced cellular death were examined in this study. In silico analysis of CBD showed antioxidant capacity via proton donation and UV absorption at 209.09, 254.73, and 276.95 nm, according to the HAT and SPLET methodologies. FS‐CBD protected against UVB‐induced bacterial death for 30 min. FS‐CBD protected against UVB‐induced cell death by 42% (1.5 μg/mL) and 35% (3.5 μg/mL) in an in vitro keratinocyte cell model. An in vivo acute irradiated CD‐1et/et mouse model (UVB‐irradiated for 5 min) presented very low photoprotection when FS‐CBD was applied cutaneously, as determined by histological analyses. In vivo skin samples showed that FS‐CBD regulated inflammatory responses by inhibiting the inflammatory markers TGF‐β1 and NLRP3. The docking analysis showed that the CBD molecule had a high affinity for TGF‐β1 and NLRP3, indicating that protection against inflammation might be mediated by blocking these proinflammatory molecules. This result was corroborated by the docking interactions between CBD and TGF‐β1 and NLRP3, which resulted in a high affinity and inhibition of both proteins The present work suggested a FS‐CBD moderate photoprotective agent against UVB light‐induced skin damage and that this effect is partially mediated by its anti‐inflammatory activity.

Publisher

Wiley

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