内吞作用
生物物理学
动力学
淀粉样蛋白(真菌学)
荧光
蛋白质聚集
生物
体内
荧光寿命成像显微镜
化学
细胞生物学
生物化学
细胞
植物
量子力学
物理
生物技术
作者
Elin K. Esbjörner,Fiona Chan,Eric J. Rees,Miklós Erdélyi,Leila M. Luheshi,Carlos W. Bertoncini,Clemens F. Kaminski,Christopher M. Dobson,Gabriele S. Kaminski Schierle
出处
期刊:Chemistry & Biology
[Elsevier]
日期:2014-05-22
卷期号:21 (6): 732-742
被引量:119
标识
DOI:10.1016/j.chembiol.2014.03.014
摘要
Insight into how amyloid β (Aβ) aggregation occurs in vivo is vital for understanding the molecular pathways that underlie Alzheimer’s disease and requires new techniques that provide detailed kinetic and mechanistic information. Using noninvasive fluorescence lifetime recordings, we imaged the formation of Aβ(1–40) and Aβ(1–42) aggregates in live cells. For both peptides, the cellular uptake via endocytosis is rapid and spontaneous. They are then retained in lysosomes, where their accumulation leads to aggregation. The kinetics of Aβ(1–42) aggregation are considerably faster than those of Aβ(1–40) and, unlike those of the latter peptide, show no detectable lag phase. We used superresolution fluorescence imaging to examine the resulting aggregates and could observe compact amyloid structures, likely because of spatial confinement within cellular compartments. Taken together, these findings provide clues as to how Aβ aggregation may occur within neurons.
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