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触发式笼状STORM显微镜技术

Triggered cagedSTORM microscopy.

作者信息

Bíró Péter, Novák Tibor, Czvik Elvira, Mihály József, Szikora Szilárd, van de Linde Sebastian, Erdélyi Miklós

机构信息

Department of Optics and Quantum Electronics, University of Szeged, Dóm tér 9, Szeged 6720, Hungary.

Institute of Genetics, HUN-REN Biological Research Centre Szeged, Temesvári körút 62, Szeged 6726, Hungary.

出版信息

Biomed Opt Express. 2024 May 15;15(6):3715-3726. doi: 10.1364/BOE.517480. eCollection 2024 Jun 1.

Abstract

In standard SMLM methods, the photoswitching of single fluorescent molecules and the data acquisition processes are independent, which leads to the detection of single molecule blinking events on several consecutive frames. This mismatch results in several data points with reduced localization precision, and it also increases the possibilities of overlapping. Here we discuss how the synchronization of the fluorophores' ON state to the camera exposure time increases the average intensity of the captured point spread functions and hence improves the localization precision. Simulations and theoretical results show that such synchronization leads to fewer localizations with 15% higher sum signal on average, while reducing the probability of overlaps by 10%.

摘要

在标准的超分辨显微镜定位方法中,单个荧光分子的光开关过程与数据采集过程是相互独立的,这导致在连续的几帧图像中检测到单分子闪烁事件。这种不匹配会导致几个定位精度降低的数据点,同时也增加了重叠的可能性。在此,我们讨论如何将荧光团的开启状态与相机曝光时间同步,以增加捕获的点扩散函数的平均强度,从而提高定位精度。模拟和理论结果表明,这种同步可使定位点减少,平均总信号提高15%,同时将重叠概率降低10%。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/a5d8/11166440/68c323349237/boe-15-6-3715-g001.jpg

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