小泡
分辨率(逻辑)
光谱分辨率
图像分辨率
化学
光谱成像
显微镜
生物物理学
光学
材料科学
物理
膜
谱线
计算机科学
生物
人工智能
生物化学
天文
作者
Yifei Jiang,Jicheng Zhang,Seung‐Ryoung Jung,Haobin Chen,Shihan Xu,Daniel T. Chiu
标识
DOI:10.1002/anie.202217889
摘要
The spatial resolution of single-molecule localization microscopy is limited by the photon number of a single switching event because of the difficulty of correlating switching events dispersed in time. Here we overcome this limitation by developing a new class of photoswitching semiconducting polymer dots (Pdots) with structured and highly dispersed single-particle spectra. We imaged the Pdots at the first and the second vibronic emission peaks and used the ratio of peak intensities as a spectral coding. By correlating switching events using the spectral coding and performing 4-9 frame binning, we achieved a 2-3 fold experimental resolution improvement versus conventional superresolution imaging. We applied this method to count and map SV2 and proton ATPase proteins on synaptic vesicles (SVs). The results reveal that these proteins are trafficked and organized with high precision, showing unprecedented level of detail about the composition and structure of SVs.
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