Delayed effects of radiation in adipose tissue reflect progenitor damage and not cellular senescence

被引:4
作者
Ruggiero, Alistaire D. [1 ]
Davis, Matthew A. [2 ]
Davis, Ashley T. [1 ]
DeStephanis, Darla [1 ]
Williams, Abigail G. [1 ]
Vemuri, Ravichandra [1 ]
Fanning, Katherine M. [1 ]
Sherrill, Chrissy [1 ]
Cline, J. Mark [1 ]
Caudell, David L. [1 ]
Kavanagh, Kylie [1 ,3 ]
机构
[1] Wake Forest Univ, Bowman Gray Sch Med, Dept Pathol, 575 N Patterson Ave, Winston Salem, NC 27101 USA
[2] Wake Forest Univ, Bowman Gray Sch Med, Dept Internal Med, Winston Salem, NC 27103 USA
[3] Univ Tasmania, Coll Hlth & Med, Hobart, Tas, Australia
基金
美国国家卫生研究院;
关键词
Radiation; Senescence; Adipose; Liver; Adipose progenitors; INSULIN-RESISTANCE; SKELETAL-MUSCLE; BRAIN-INJURY; IRRADIATION; EXPOSURE; GAMMA; DYSFUNCTION; EXPRESSION; BIOMARKER; DISEASE;
D O I
10.1007/s11357-022-00660-x
中图分类号
R592 [老年病学]; C [社会科学总论];
学科分类号
03 ; 0303 ; 100203 ;
摘要
The pathogenesis of many age-related diseases is linked to cellular senescence, a state of inflammation-inducing, irreversible cell cycle arrest. The consequences and mechanisms of age-associated cellular senescence are often studied using in vivo models of radiation exposure. However, it is unknown whether radiation induces persistent senescence, like that observed in ageing. We performed analogous studies in mice and monkeys, where young mice and rhesus macaques received sub-lethal doses of ionizing radiation and were observed for similar to 15% of their expected lifespan. Assessments of 8-hydroxy-2' - deoxyguanosine (8-OHdG), senescence-associated beta-galactosidase (SA beta-gal), and p16(Ink4)(a) and p21 were performed on mitotic and post-mitotic tissues - liver and adipose tissue - 6 months and 3 years post-exposure for the mice and monkeys, respectively. No elevations in 8-OHdG, SA-beta gal staining, or p16(Ink4a) or p21 gene or protein expression were found in mouse and monkey liver or adipose tissue compared to control animals. Despite no evidence of senescence, progenitor cell dysfunction persisted after radiation exposure, as indicated by lower in situ CD34(+) adipose cells (p = 0 .03) , and deficient adipose stromal vascular cell proliferation (p <0.05) and differentiation (p = 0.04) ex vivo. Our investigation cautions that employing radiation to study senescence-related processes should be limited to the acute post-exposure period and that stem cell damage likely underpins the dysfunction associated with delayed effects of radiation.
引用
收藏
页码:507 / 521
页数:15
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