The mechanism of internalization study of QDgreen−CD−FA−C−2028 conjugate at IC80 value to cancer (H460, Du-145, and LNCaP) and normal (MRC-5 and PNT1A) cells
Description
The influence of different endocytosis inhibitors on the internalization of QDgreen−CD−FA−C−2028 conjugate at IC80 value in cancer (H460, Du-145, and LNCaP) and normal (MRC-5 and PNT1A) cells. First, the cells were preincubated with: drug-free medium (no inhibitor), at 4 °C, 5 µM Cytochalasin D, 30 µM Amiloride, 80 µM Dynasore, 25 µM Pitstop 2 and 1.5 µM Filipin III for 30 min, followed by further incubation with QDgreen−CD−FA−C−2028 for 4 h. The internalization of QDgreen−CD−FA−C−2028 in cells was explored by Confocal Laser Scanning Microscopy (63× magnification; ZEISS LSM T-PMT). Based on the fluorescence properties of these compounds, green and orange fluorescence are representative for QDgreen and C−2028, respectively. The imaging conditions were: QDgreen (excitation 300 nm, emission 543 nm), C−2028 (excitation 528 nm, emission 553 nm). The scale bar is 20 μm.
Dataset file
hexmd5(md5(part1)+md5(part2)+...)-{parts_count}
where a single part of the file is 512 MB in size.Example script for calculation:
https://github.com/antespi/s3md5
File details
- License:
-
open in new tabCC BY-NC-SANon-commercial - Share-alike
Details
- Year of publication:
- 2021
- Verification date:
- 2021-12-09
- Dataset language:
- English
- Fields of science:
-
- chemical sciences (Natural sciences)
- biomedical engineering (Engineering and Technology)
- DOI:
- DOI ID 10.34808/zsy0-az13 open in new tab
- Funding:
- Verified by:
- Gdańsk University of Technology
Keywords
- endocytosis inhibitors
- internalization
- cellular uptake
- confocal microscopy
- nanoparticles
- unsymmetrical bisacridines
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