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Bioluminescence Imaging with Functional Amyloid Reservoirs in Alzheimer’s Disease Models

生物发光 生物发光成像 荧光素酶 体内 化学 临床前影像学 淀粉样蛋白(真菌学) 生物物理学 转基因小鼠 阿尔茨海默病 转基因 病理 生物化学 生物 疾病 医学 基因 生物技术 无机化学 转染
作者
Jing Yang,Weihua Ding,Biyue Zhu,Sherri Zhen,Shi Kuang,Jun Yang,Can Zhang,Peng Wang,Fan Yang,Liuyue Yang,Wei Yin,Rudolph E. Tanzi,Shiqian Shen,Chongzhao Ran
出处
期刊:Analytical Chemistry [American Chemical Society]
卷期号:95 (38): 14261-14270 被引量:2
标识
DOI:10.1021/acs.analchem.3c02358
摘要

Bioluminescence imaging has changed the daily practice of preclinical research on cancer and other diseases over the last few decades; however, it has rarely been applied in preclinical research on Alzheimer's disease (AD). In this Article, we demonstrated that bioluminescence imaging could be used to report the levels of amyloid beta (Aβ) species in vivo. We hypothesized that AkaLumine, a newly discovered substrate for luciferase, could bind to Aβ aggregates and plaques. We further speculated that the Aβ aggregates/fibrils/plaques could be considered as "functional amyloids", which have a reservoir function to sequester and release AkaLumine to control the bioluminescence intensity, which could be used to report the levels of Aβs. Our hypotheses have been validated via in vitro solution tests, mimic studies with brain tissues and mice, two-photon imaging with AD mice, and in vivo bioluminescence imaging using transgenic AD mice that were virally transduced with AkaLuciferase (AkaLuc), a new luciferase that generates bioluminescence in the near-infrared window. As expected, compared to the control group, we observed that the Aβ group showed lower bioluminescence intensity due to AkaLumine sequestering at early time points, while higher intensity was due to AkaLumine releasing at later time points. Lastly, we demonstrated that this method could be used to monitor AD progression and the therapeutic effectiveness of avagacestat, a well-studied gamma-secretase inhibitor. Importantly, a good correlation (R2 = 0.81) was established between in vivo bioluminescence signals and Aβ burdens of the tested AD mice. We believe that our approach can be easily implemented into daily imaging experiments and has tremendous potential to change the daily practice of preclinical AD research.
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