Article ? AI-assigned paper type based on the abstract. Classification may not be perfect — flag errors using the feedback button. Tier 2 ? Original research — experimental, observational, or case-control study. Direct primary evidence. Environmental Sources Human Health Effects Nanoplastics Policy & Risk Reproductive & Development Sign in to save

Polystyrene nanoplastics exposure triggers spermatogenic cell senescence via the Sirt1/ROS axis

Ecotoxicology and Environmental Safety 2024 29 citations ? Citation count from OpenAlex, updated daily. May differ slightly from the publisher's own count. Score: 65 ? 0–100 AI score estimating relevance to the microplastics field. Papers below 30 are filtered from public browse.

Yuehui Liang, Yuehui Liang, Yuehui Liang, Chunsheng Lu, Yurui Yang, Yurui Yang, Yuehui Liang, Yuehui Liang, Chunsheng Lu, Ya Cheng, Ya Cheng, Jia Cao, Qing Chen, Xiao Jiang, Xiao Jiang, Qing Chen, Jinyi Liu, Qing Chen, Binwei Yang, Yuehui Liang, Yuehui Liang, Binwei Yang, Yuehui Liang, Fei Han Yuehui Liang, Yawen Li, Yuehui Liang, Fei Han Xiao Jiang, Qing Chen, Xiao Jiang, Lin Ao, Lin Ao, Xiao Jiang, Jia Cao, Fei Han Jinyi Liu, Fei Han Jia Cao, Fei Han Chunsheng Lu, Jinyi Liu, Lina Zhao, Fei Han Fei Han

Summary

Male mice exposed to polystyrene nanoplastics for 60 days showed damaged sperm-producing cells that displayed signs of premature aging, linked to a specific molecular pathway involving the Sirt1 protein and oxidative stress. This study adds to growing evidence that nanoplastic exposure may harm male reproductive health by accelerating the aging of cells responsible for sperm production.

Polymers

Body Systems

Reproductive

Models

Mouse

Study Type In vivo

Polystyrene nanoplastics (PS-NPs) have been reported to accumulate in the testes and constitute a new threat to reproductive health. However, the exact effects of PS-NPs exposure on testicular cells and the underlying mechanisms remain largely unknown. The C57BL/6 male mice were orally administered with PS-NPs (80 nm) at different dosages (0, 10, and 40 mg/kg/day) for 60 days, and GC-1 cells were treated with PS-NPs in this study. Enlarged seminiferous tubule lumens and a loose and vacuolated layer of spermatogenic cells were observed in PS-NPs-exposed mice. Spermatogenic cells which may be one of the target cells for this reproductive damage, were decreased in the mice from PS-NPs group. PS-NPs caused spermatogenic cells to undergo senescence, manifested as elevated SA-β-galactosidase activity and activated senescence-related signaling p53-p21/Rb-p16 pathways, and induced cell cycle arrest. Mechanistically, Gene Ontology (GO) enrichment suggested the key role of reactive oxygen species (ROS) in PS-NPs-induced spermatogenic cell senescence, and this result was confirmed by measuring ROS levels. Moreover, ROS inhibition partially attenuated the senescence phenotype of spermatogenic cells and DNA damage. Using the male health atlas (MHA) database, Sirt1 was filtrated as the critical molecule in the regulation of testicular senescence. PS-NPs induced overexpression of the main ROS generator Nox2, downregulated Sirt1, increased p53 and acetylated p53 in vivo and in vitro, whereas these disturbances were partially restored by pterostilbene. In addition, pterostilbene intervention significantly alleviated the PS-NPs-induced spermatogenic cell senescence and attenuated ROS burst. Collectively, our study reveals that PS-NPs exposure can trigger spermatogenic cell senescence mediated by p53-p21/Rb-p16 signaling by regulating the Sirt1/ROS axis. Importantly, pterostilbene intervention may be a promising strategy to alleviate this damage.

Read via DOI Download PDF

Share this paper

Post Share Share Pin Email