Discovery of an Ultra‐rapid and Sensitive Lysosomal Fluorescence Lipophagy Process
Non‐invasive dynamic tracking of lysosomes and their interactions with other organelles is important for the study of lysosomal function and related diseases. However, many fluorescent dyes developed so far to target lysosomes cannot be used to monitor these processes due to the high concentrations...
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| Vydané v: | Angewandte Chemie International Edition Ročník 61; číslo 11; s. e202116439 - n/a |
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| Hlavní autori: | , , , , , , , , , , , , |
| Médium: | Journal Article |
| Jazyk: | English |
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WEINHEIM
Wiley
07.03.2022
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| Vydanie: | International ed. in English |
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| ISSN: | 1433-7851, 1521-3773, 1521-3773 |
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| Abstract | Non‐invasive dynamic tracking of lysosomes and their interactions with other organelles is important for the study of lysosomal function and related diseases. However, many fluorescent dyes developed so far to target lysosomes cannot be used to monitor these processes due to the high concentrations required for imaging, long cell penetration times, and non‐ideal photostability. In this regard, we synthesized three lysosomal targeting probes with large Stokes shifts, good stability, and high brightness. The Q‐P‐ARh dye, developed by us for the first time, can stain lysosomes at ultra‐low concentrations (1.0 nM) without affecting the physiological functions of the lysosomes. More importantly, its excellent anti‐interference ability and ultrafast lysosomal staining ability (within 1.0 min) clearly monitored the entire dynamic process of lipophagy. Ultimately, this method can greatly contribute to the study of autophagy pathways. This novel fluorescence platform shows great promise for the development of biological probes for application in pathological environments.
A series of brand‐new large Stokes shift and highly stable fluorescent dyes were constructed. In particular, the Q‐P‐ARh fluorescent dye as a near‐infrared emission lysosomal‐specific probe with ultra‐low concentration and ultra‐fast staining characteristics for the complete lipophagy process imaging is presented. |
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| AbstractList | Non‐invasive dynamic tracking of lysosomes and their interactions with other organelles is important for the study of lysosomal function and related diseases. However, many fluorescent dyes developed so far to target lysosomes cannot be used to monitor these processes due to the high concentrations required for imaging, long cell penetration times, and non‐ideal photostability. In this regard, we synthesized three lysosomal targeting probes with large Stokes shifts, good stability, and high brightness. The Q‐P‐ARh dye, developed by us for the first time, can stain lysosomes at ultra‐low concentrations (1.0 nM) without affecting the physiological functions of the lysosomes. More importantly, its excellent anti‐interference ability and ultrafast lysosomal staining ability (within 1.0 min) clearly monitored the entire dynamic process of lipophagy. Ultimately, this method can greatly contribute to the study of autophagy pathways. This novel fluorescence platform shows great promise for the development of biological probes for application in pathological environments.
A series of brand‐new large Stokes shift and highly stable fluorescent dyes were constructed. In particular, the Q‐P‐ARh fluorescent dye as a near‐infrared emission lysosomal‐specific probe with ultra‐low concentration and ultra‐fast staining characteristics for the complete lipophagy process imaging is presented. Non-invasive dynamic tracking of lysosomes and their interactions with other organelles is important for the study of lysosomal function and related diseases. However, many fluorescent dyes developed so far to target lysosomes cannot be used to monitor these processes due to the high concentrations required for imaging, long cell penetration times, and non-ideal photostability. In this regard, we synthesized three lysosomal targeting probes with large Stokes shifts, good stability, and high brightness. The Q-P-ARh dye, developed by us for the first time, can stain lysosomes at ultra-low concentrations (1.0 nM) without affecting the physiological functions of the lysosomes. More importantly, its excellent anti-interference ability and ultrafast lysosomal staining ability (within 1.0 min) clearly monitored the entire dynamic process of lipophagy. Ultimately, this method can greatly contribute to the study of autophagy pathways. This novel fluorescence platform shows great promise for the development of biological probes for application in pathological environments. Non-invasive dynamic tracking of lysosomes and their interactions with other organelles is important for the study of lysosomal function and related diseases. However, many fluorescent dyes developed so far to target lysosomes cannot be used to monitor these processes due to the high concentrations required for imaging, long cell penetration times, and non-ideal photostability. In this regard, we synthesized three lysosomal targeting probes with large Stokes shifts, good stability, and high brightness. The Q-P-ARh dye, developed by us for the first time, can stain lysosomes at ultra-low concentrations (1.0 nM) without affecting the physiological functions of the lysosomes. More importantly, its excellent anti-interference ability and ultrafast lysosomal staining ability (within 1.0 min) clearly monitored the entire dynamic process of lipophagy. Ultimately, this method can greatly contribute to the study of autophagy pathways. This novel fluorescence platform shows great promise for the development of biological probes for application in pathological environments.Non-invasive dynamic tracking of lysosomes and their interactions with other organelles is important for the study of lysosomal function and related diseases. However, many fluorescent dyes developed so far to target lysosomes cannot be used to monitor these processes due to the high concentrations required for imaging, long cell penetration times, and non-ideal photostability. In this regard, we synthesized three lysosomal targeting probes with large Stokes shifts, good stability, and high brightness. The Q-P-ARh dye, developed by us for the first time, can stain lysosomes at ultra-low concentrations (1.0 nM) without affecting the physiological functions of the lysosomes. More importantly, its excellent anti-interference ability and ultrafast lysosomal staining ability (within 1.0 min) clearly monitored the entire dynamic process of lipophagy. Ultimately, this method can greatly contribute to the study of autophagy pathways. This novel fluorescence platform shows great promise for the development of biological probes for application in pathological environments. Non‐invasive dynamic tracking of lysosomes and their interactions with other organelles is important for the study of lysosomal function and related diseases. However, many fluorescent dyes developed so far to target lysosomes cannot be used to monitor these processes due to the high concentrations required for imaging, long cell penetration times, and non‐ideal photostability. In this regard, we synthesized three lysosomal targeting probes with large Stokes shifts, good stability, and high brightness. The Q‐P‐ARh dye, developed by us for the first time, can stain lysosomes at ultra‐low concentrations (1.0 nM) without affecting the physiological functions of the lysosomes. More importantly, its excellent anti‐interference ability and ultrafast lysosomal staining ability (within 1.0 min) clearly monitored the entire dynamic process of lipophagy. Ultimately, this method can greatly contribute to the study of autophagy pathways. This novel fluorescence platform shows great promise for the development of biological probes for application in pathological environments. |
| ArticleNumber | 202116439 |
| Author | Won, Miae Zhang, Hong Li, Kun Kim, Jong Seung Liu, Yan‐Hong Choe, Youmi Yu, Xiao‐Qi Liu, Yan‐Zhao Shi, Lei Chen, Shan‐Yong Liu, Xin Liu, Xin‐Yao Yu, Kang‐Kang |
| Author_xml | – sequence: 1 givenname: Hong surname: Zhang fullname: Zhang, Hong organization: Sichuan University – sequence: 2 givenname: Lei surname: Shi fullname: Shi, Lei organization: Sichuan University – sequence: 3 givenname: Kun orcidid: 0000-0002-8788-1036 surname: Li fullname: Li, Kun email: kli@scu.edu.cn organization: Sichuan University – sequence: 4 givenname: Xin surname: Liu fullname: Liu, Xin organization: Sichuan University – sequence: 5 givenname: Miae orcidid: 0000-0002-1656-6362 surname: Won fullname: Won, Miae organization: Korea University – sequence: 6 givenname: Yan‐Zhao surname: Liu fullname: Liu, Yan‐Zhao organization: Sichuan University – sequence: 7 givenname: Youmi surname: Choe fullname: Choe, Youmi organization: Korea University – sequence: 8 givenname: Xin‐Yao surname: Liu fullname: Liu, Xin‐Yao organization: Sichuan University – sequence: 9 givenname: Yan‐Hong surname: Liu fullname: Liu, Yan‐Hong organization: Sichuan University – sequence: 10 givenname: Shan‐Yong surname: Chen fullname: Chen, Shan‐Yong organization: Sichuan University – sequence: 11 givenname: Kang‐Kang surname: Yu fullname: Yu, Kang‐Kang organization: Sichuan University – sequence: 12 givenname: Jong Seung orcidid: 0000-0003-3477-1172 surname: Kim fullname: Kim, Jong Seung email: jongskim@korea.ac.kr organization: Korea University – sequence: 13 givenname: Xiao‐Qi orcidid: 0000-0003-1719-6137 surname: Yu fullname: Yu, Xiao‐Qi email: xqyu@scu.edu.cn organization: Sichuan University |
| BackLink | https://www.ncbi.nlm.nih.gov/pubmed/34964238$$D View this record in MEDLINE/PubMed |
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| CitedBy_id | crossref_primary_10_1016_j_ccr_2023_215203 crossref_primary_10_1039_D4MH00190G crossref_primary_10_1002_chem_202301073 crossref_primary_10_1039_D5MH01254F crossref_primary_10_1002_agt2_708 crossref_primary_10_1039_D5NJ01958C crossref_primary_10_1055_a_2201_3612 crossref_primary_10_1039_D4SD00038B crossref_primary_10_1016_j_bios_2023_115707 crossref_primary_10_3390_bios15060383 crossref_primary_10_1002_adfm_202412595 crossref_primary_10_1021_acs_analchem_5c01619 crossref_primary_10_1002_adhm_202402295 crossref_primary_10_1016_j_jhazmat_2023_133106 crossref_primary_10_1002_adma_202503220 crossref_primary_10_1002_anie_202301598 crossref_primary_10_1002_ange_202301598 crossref_primary_10_1002_adma_202210179 crossref_primary_10_1016_j_bios_2024_116084 crossref_primary_10_1039_D4MH01167H |
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| Keywords | CELLS ADIPOCYTES DYES Lipophagy Large Stokes Shift Lysosomes AUTOPHAGY DIFFERENTIATION MODEL Near-Infrared PROBES |
| Language | English |
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| SubjectTerms | Autophagy Chemistry Chemistry, Multidisciplinary Dyes Fluorescence Fluorescent dyes Fluorescent indicators Large Stokes Shift Lipophagy Low concentrations Lysosomes Near-Infrared Organelles Physical Sciences Probes Science & Technology |
| Title | Discovery of an Ultra‐rapid and Sensitive Lysosomal Fluorescence Lipophagy Process |
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