An Ex Vivo Aorta Culture Model to Study Vascular Cellular Senescence

Author:

Yu Yijie1,Bian Shihui2,Jiang Yu1,Li Bo1,Cui Xinggang1,Ding Shu1,Dai Zhiyin1,Chen Rui1,Zhong Wei1ORCID,Yuan Wei1

Affiliation:

1. Department of Cardiology Affiliated Hospital of Jiangsu University Zhenjiang Jiangsu P. R. China

2. Department of Geriatrics Affiliated People's Hospital of Jiangsu University Zhenjiang Jiangsu P. R. China

Abstract

AbstractAnimal studies on vascular aging pose a few limitations. One of the most important reasons for this is the absence of a fast and efficient model of vascular tissue aging. In this study, ex vivo aortic culture and Matrigel subcutaneous implantation are combined to develop a new model for studying vascular cellular senescence. Eight‐week‐old C57BL/6J mice are used to obtain aortas. Bleomycin is used to induce aortas senescence in vitro. Then, aortas are transplanted to the acceptor mice with Matrigel. Senescence is evaluated using western blotting, quantitative polymerase chain reaction, and senescence‐associated beta‐galactosidase activity. Inflammatory cytokines are detected using Luminex Liquid Suspension Chip. RNA levels are analyzed by transcriptome sequencing. The results revealed that vessels in the bleomycin group exhibited significant senescence than those in the control group that can be enhanced by stripping vessel adventitia. The levels of cytokines such as interleukin (IL‐2, IL‐1β, and IL‐6 increased significantly in the ex vivo model. Furthermore, transcriptome sequencing revealed 56 significantly differentially expressed genes (DEGs) in ex vivo model vessels compared with those in naturally aging aortas. In conclusion, this study introduces a cost‐effective and time‐saving vessel senescence model for vascular cellular senescence.

Funder

Natural Science Foundation of Jilin Province

Publisher

Wiley

Subject

General Medicine

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