4.8 Article

Aggregation-Induced Emission (AIE) in Super- resolution Imaging: Cationic AIE Luminogens (AIEgens) for Tunable Organelle-Specific Imaging and Dynamic Tracking in Nanometer Scale

ACS NANO (2022)

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Journal

ACS NANO
Volume 16, Issue 4, Pages 5932-5942

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/acsnano.1c11125

Keywords

aggregation-induced emission; anion− ir(+) interactions; super-resolution imaging; organelle-specific imaging; dynamic tracking

Categories

Chemistry, Multidisciplinary Chemistry, Physical Nanoscience & Nanotechnology Materials Science, Multidisciplinary

Funding

  1. National Natural Science Foundation of China [21975197]
  2. Fundamental Fund of Xi'an Jiao Tong University [xzy022020015]
  3. Key Laboratory Construction Program of Xi'an Municipal Bureau of Science and Technology [201805056ZD7CG40]
  4. Innovation Capability Support Program of Shaanxi [2021TD-57]
  5. Innovation and Technology Commission [ITC-CNERC14SC01]

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This study proposes a facile strategy to construct an aggregation-induced emission luminogen (AIEgen) for organelle-specific imaging and dynamic tracking. Super-resolution imaging is achieved via STED nanoscopy, allowing for high-resolution imaging and specific targeting of mitochondria and nucleus.
Organelle-specific imaging and dynamic tracking in ultrahigh resolution is essential for understanding their functions in biological research, but this remains a challenge. Therefore, a facile strategy by utilizing anion-pi+ interactions is proposed here to construct an aggregation-induced emission luminogen (AIEgen) of DTPAP-P, not only restricting the intramolecular motions but also blocking their strong pi-pi interactions. DTPAP-P exhibits a high photoluminescence quantum yield (PLQY) of 35.04% in solids, favorable photostability and biocompatibility, indicating its potential application in super-resolution imaging (SRI) via stimulated emission depletion (STED) nanoscopy. It is also observed that this cationic DTPAP-P can specifically target to mitochondria or nucleus dependent on the cell status, resulting in tunable organelle-specific imaging in nanometer scale. In live cells, mitochondria-specific imaging and their dynamic monitoring (fission and fusion) can be obtained in ultrahigh resolution with a full-width-at-half-maximum (fwhm) value of only 165 nm by STED nanoscopy. This is about one-sixth of the fwhm value in confocal microscopy (1028 nm). However, a migration process occurs for fixed cells from mitochondria to nucleus under light activation (405 nm), leading to nucleus-targeted super-resolution imaging (fwhm= 184 nm). These findings indicate that tunable organelle-specific imaging and dynamic tracking by a single AIEgen at a superior resolution can be achieved in our case here via STED nanoscopy, thus providing an efficient method to further understand organelle's functions and roles in biological research.

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