TY - JOUR
T1 - SOFISM
T2 - Super-resolution optical fluctuation image scanning microscopy
AU - Sroda, Aleksandra
AU - Makowski, Adrian
AU - Tenne, Ron
AU - Rossman, Uri
AU - Lubin, Gur
AU - Oron, Dan
AU - Lapkiewicz, Radek
N1 - Funding. European Research Council (ColloQuantO); Crown Photonics Center; Minerva Foundation; KLA-TENCOR Corporation; Narodowe Centrum Nauki (2015/17/D/ST2/ 03471); Ministerstwo Nauki i Szkolnictwa Wyższego; Foundation for Polish Science under the FIRST TEAM project ‘Spatiotemporal photon correlation measurements for quantum metrology and super-resolution microscopy’ co-financed by the European Union under the European Regional Development Fund (POIR.04.04.00-00-3004/17-00). The authors thank Y. Ebenstein for the preparation of biological samples, S. Itzhakov for synthesizing the quantum dots used in this work, and W. Kondrusiewicz, M. Pawłowska, J. Oracz, A. Krupinski-Ptaszek, and P. Fita for discussions about the work and the paper.
PY - 2020/9/29
Y1 - 2020/9/29
N2 - Super-resolution optical microscopy is a rapidly evolving scientific field dedicated to imaging sub-wavelength-sized objects, leaving its mark in multiple branches of biology and technology. While several super-resolution optical microscopy methods have become a common tool in life science imaging, new methods, supported by cutting-edge technology, continue to emerge. One rather recent addition to the super-resolution toolbox, image scanning microscopy (ISM), achieves up to twofold lateral resolution enhancement in a robust and straightforward manner. To further enhance ISM's resolution in all three dimensions, we present and experimentally demonstrate here super-resolution optical fluctuation ISM (SOFISM). Measuring the fluorescence fluctuation contrast in an ISM architecture, we obtain images with a ×2.5 lateral resolution beyond the diffraction limit along with an enhanced axial resolution for a fixed cell sample labeled with commercially available quantum dots. The inherent temporal averaging of the ISM technique enables image acquisition of the fluctuation correlation contrast within millisecond-scale pixel dwell times. SOFISM can therefore offer a robust path to achieve high-resolution images within a slightly modified confocal microscope, using standard fluorescent labels and reasonable acquisition times.
AB - Super-resolution optical microscopy is a rapidly evolving scientific field dedicated to imaging sub-wavelength-sized objects, leaving its mark in multiple branches of biology and technology. While several super-resolution optical microscopy methods have become a common tool in life science imaging, new methods, supported by cutting-edge technology, continue to emerge. One rather recent addition to the super-resolution toolbox, image scanning microscopy (ISM), achieves up to twofold lateral resolution enhancement in a robust and straightforward manner. To further enhance ISM's resolution in all three dimensions, we present and experimentally demonstrate here super-resolution optical fluctuation ISM (SOFISM). Measuring the fluorescence fluctuation contrast in an ISM architecture, we obtain images with a ×2.5 lateral resolution beyond the diffraction limit along with an enhanced axial resolution for a fixed cell sample labeled with commercially available quantum dots. The inherent temporal averaging of the ISM technique enables image acquisition of the fluctuation correlation contrast within millisecond-scale pixel dwell times. SOFISM can therefore offer a robust path to achieve high-resolution images within a slightly modified confocal microscope, using standard fluorescent labels and reasonable acquisition times.
UR - http://www.scopus.com/inward/record.url?scp=85092289296&partnerID=8YFLogxK
U2 - 10.1364/OPTICA.399600
DO - 10.1364/OPTICA.399600
M3 - مقالة
SN - 2334-2536
VL - 7
SP - 1308
EP - 1316
JO - Optica
JF - Optica
IS - 10
ER -