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A new organic molecular probe as a powerful tool for fluorescence imaging and biological study of lipid droplets

Background: Lipid droplets (LDs) are critical organelles associated with many physiological processes in eukaryotic cells. To visualize and study LDs, fluorescence imaging techniques including the confocal imaging as well as the emerging super-resolution imaging of stimulated emission depletion (STE...

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Autores principales: Zhou, Ri, Wang, Chenguang, Liang, Xishuang, Liu, Fangmeng, Sun, Peng, Yan, Xu, Jia, Xiaoteng, Liu, Xiaomin, Wang, Yue, Lu, Geyu
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Ivyspring International Publisher 2023
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9800742/
https://www.ncbi.nlm.nih.gov/pubmed/36593956
http://dx.doi.org/10.7150/thno.79052
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author Zhou, Ri
Wang, Chenguang
Liang, Xishuang
Liu, Fangmeng
Sun, Peng
Yan, Xu
Jia, Xiaoteng
Liu, Xiaomin
Wang, Yue
Lu, Geyu
author_facet Zhou, Ri
Wang, Chenguang
Liang, Xishuang
Liu, Fangmeng
Sun, Peng
Yan, Xu
Jia, Xiaoteng
Liu, Xiaomin
Wang, Yue
Lu, Geyu
author_sort Zhou, Ri
collection PubMed
description Background: Lipid droplets (LDs) are critical organelles associated with many physiological processes in eukaryotic cells. To visualize and study LDs, fluorescence imaging techniques including the confocal imaging as well as the emerging super-resolution imaging of stimulated emission depletion (STED), have been regarded as the most useful methods. However, directly limited by the availability of advanced LDs fluorescent probes, the performances of LDs fluorescence imaging are increasingly unsatisfied with respect to the fast research progress of LDs. Methods: We herein newly developed a superior LDs fluorescent probe named Lipi-QA as a powerful tool for LDs fluorescence imaging and biological study. Colocalization imaging of Lipi-QA and LDs fluorescent probe Ph-Red was conducted in four cell lines. The LDs staining selectivity and the photostability of Lipi-QA were also evaluated by comparing with the commercial LDs probe Nile Red. The in-situ fluorescence lifetime of Lipi-QA in LDs was determined by time-gated detection. The cytotoxicity of Lipi-QA was assessed by MTT assay. The STED saturation intensity as well as the power- and gate time-dependent resolution were tested by Leica SP8 STED super-resolution nanoscopy. The time-lapse 3D confocal imaging and time-lapse STED super-resolution imaging were then designed to study the complex physiological functions of LDs. Results: Featuring with the advantages of the super-photostability, high LDs selectivity, long fluorescence lifetime and low STED saturation intensity, the fluorescent probe Lipi-QA was capable of the long-term time-lapse three-dimensional (3D) confocal imaging to in-situ monitor LDs in 3D space and the time-lapse STED super-resolution imaging (up to 500 STED frames) to track the dynamics of LDs with nanoscale resolution (37 nm). Conclusions: Based on the state-of-the-art fluorescence imaging results, some new biological insights into LDs have been successfully provided. For instance, the long-term time-lapse 3D confocal imaging has surely answered an important and controversial question that the number of LDs would significantly decrease rather than increase upon starvation stimulation; the time-lapse STED super-resolution imaging with the highest resolution has impressively uncovered the fission process of nanoscale LDs for the first time; the starvation-induced change of LDs in size and in speed has been further revealed at nanoscale by the STED super-resolution imaging. All of these results not only highlight the utility of the newly developed fluorescent probe but also significantly promote the biological study of LDs.
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spelling pubmed-98007422023-01-01 A new organic molecular probe as a powerful tool for fluorescence imaging and biological study of lipid droplets Zhou, Ri Wang, Chenguang Liang, Xishuang Liu, Fangmeng Sun, Peng Yan, Xu Jia, Xiaoteng Liu, Xiaomin Wang, Yue Lu, Geyu Theranostics Research Paper Background: Lipid droplets (LDs) are critical organelles associated with many physiological processes in eukaryotic cells. To visualize and study LDs, fluorescence imaging techniques including the confocal imaging as well as the emerging super-resolution imaging of stimulated emission depletion (STED), have been regarded as the most useful methods. However, directly limited by the availability of advanced LDs fluorescent probes, the performances of LDs fluorescence imaging are increasingly unsatisfied with respect to the fast research progress of LDs. Methods: We herein newly developed a superior LDs fluorescent probe named Lipi-QA as a powerful tool for LDs fluorescence imaging and biological study. Colocalization imaging of Lipi-QA and LDs fluorescent probe Ph-Red was conducted in four cell lines. The LDs staining selectivity and the photostability of Lipi-QA were also evaluated by comparing with the commercial LDs probe Nile Red. The in-situ fluorescence lifetime of Lipi-QA in LDs was determined by time-gated detection. The cytotoxicity of Lipi-QA was assessed by MTT assay. The STED saturation intensity as well as the power- and gate time-dependent resolution were tested by Leica SP8 STED super-resolution nanoscopy. The time-lapse 3D confocal imaging and time-lapse STED super-resolution imaging were then designed to study the complex physiological functions of LDs. Results: Featuring with the advantages of the super-photostability, high LDs selectivity, long fluorescence lifetime and low STED saturation intensity, the fluorescent probe Lipi-QA was capable of the long-term time-lapse three-dimensional (3D) confocal imaging to in-situ monitor LDs in 3D space and the time-lapse STED super-resolution imaging (up to 500 STED frames) to track the dynamics of LDs with nanoscale resolution (37 nm). Conclusions: Based on the state-of-the-art fluorescence imaging results, some new biological insights into LDs have been successfully provided. For instance, the long-term time-lapse 3D confocal imaging has surely answered an important and controversial question that the number of LDs would significantly decrease rather than increase upon starvation stimulation; the time-lapse STED super-resolution imaging with the highest resolution has impressively uncovered the fission process of nanoscale LDs for the first time; the starvation-induced change of LDs in size and in speed has been further revealed at nanoscale by the STED super-resolution imaging. All of these results not only highlight the utility of the newly developed fluorescent probe but also significantly promote the biological study of LDs. Ivyspring International Publisher 2023-01-01 /pmc/articles/PMC9800742/ /pubmed/36593956 http://dx.doi.org/10.7150/thno.79052 Text en © The author(s) https://creativecommons.org/licenses/by/4.0/This is an open access article distributed under the terms of the Creative Commons Attribution License (https://creativecommons.org/licenses/by/4.0/). See http://ivyspring.com/terms for full terms and conditions.
spellingShingle Research Paper
Zhou, Ri
Wang, Chenguang
Liang, Xishuang
Liu, Fangmeng
Sun, Peng
Yan, Xu
Jia, Xiaoteng
Liu, Xiaomin
Wang, Yue
Lu, Geyu
A new organic molecular probe as a powerful tool for fluorescence imaging and biological study of lipid droplets
title A new organic molecular probe as a powerful tool for fluorescence imaging and biological study of lipid droplets
title_full A new organic molecular probe as a powerful tool for fluorescence imaging and biological study of lipid droplets
title_fullStr A new organic molecular probe as a powerful tool for fluorescence imaging and biological study of lipid droplets
title_full_unstemmed A new organic molecular probe as a powerful tool for fluorescence imaging and biological study of lipid droplets
title_short A new organic molecular probe as a powerful tool for fluorescence imaging and biological study of lipid droplets
title_sort new organic molecular probe as a powerful tool for fluorescence imaging and biological study of lipid droplets
topic Research Paper
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC9800742/
https://www.ncbi.nlm.nih.gov/pubmed/36593956
http://dx.doi.org/10.7150/thno.79052
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