研究目的
Investigating the pharmacologic effect on cellular processes and the potential toxicological effects of new drug development and evaluation through visualizing the spatiotemporal distribution of drugs and metabolites within a single cell.
研究成果
The study demonstrated the potential of NDPI-MS for single-cell imaging of structurally similar acridine drugs, revealing concentration-dependent intracellular distribution and drug accumulation at the organelle level. The findings highlight the importance of considering drug distribution within cells beyond plasma concentration and the utility of high-resolution MSI in drug discovery and development.
研究不足
The study acknowledges the challenge of direct visualization of cytoplasmic organelles due to the limited detection sensitivity of endogenous markers. Additionally, the complexity of the intracellular environment may affect the luminescence of drugs, potentially leading to misleading results when using a single characterization technique.
1:Experimental Design and Method Selection:
The study utilized near-field laser desorption/laser postionization mass spectrometry (NDPI-MS) for single-cell imaging of two structurally similar drugs, proflavine and ethacridine. The methodology included high spatial resolution by near-field desorption and high ionization efficiency by single-photon postionization.
2:Sample Selection and Data Sources:
HeLa cells were used as the biological sample, treated with proflavine and ethacridine at various concentrations. The cells were fixed and prepared for MSI and LSCM imaging.
3:List of Experimental Equipment and Materials:
The NDPI-MS system included a desorption laser, a nanoscale aperture fiber probe, a modified atomic force microscope (AFM) system, a high-precision nanopositioner, and a 157 nm F2 laser for postionization. Chemicals included proflavine hydrochloride, ethacridine lactate, and LysoTracker? Blue.
4:Experimental Procedures and Operational Workflow:
Cells were treated with drugs, fixed, and imaged using NDPI-MS and LSCM. The NDPI-MS imaging was performed with a 250 nm step size and one laser pulse per pixel.
5:Data Analysis Methods:
The generated ions were detected by TOFMS, and the MSI of drug distribution was acquired through pixel-by-pixel scanning. Correlated NDPI and LSCM imaging were used to confirm drug accumulation locations.
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Laser scanning confocal microscope
TCS SP5
Leica Microsystems
Used for fluorescence imaging of drugs and DND-22.
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Atomic force microscope
MadPLL
Mad City Lab. Inc.
Used for precisely controlling the distance between the aperture tip and the sample surface.
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Nanopositioner
SLC-17
SmartAct GmbH
Used for sample scanning in NDPI-MS.
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F2 laser
ExciStar XS 200
Coherent Inc.
Used for postionization in NDPI-MS.
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Digital oscilloscope
42MXs
LeCroy
Used for recording the mass spectral signals in NDPI-MS.
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Proflavine hydrochloride
Sigma-Aldrich
Used as a chemotherapeutic agent for neurological diseases and cancers.
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Ethacridine lactate
Shanghai Aladdin Biochemical Technology Co., Ltd.
Used as an antibacterial agent.
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Dulbecco’s modified Eagle’s medium
HyClone
Culture medium for HeLa cells.
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Fetal bovine serum
Sigma-Aldrich
Supplement for cell culture medium.
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LysoTracker? Blue
DND-22
Xiamen Bioluminor Bio-Tech Co., Ltd.
Stains lysosomes with high specificity.
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Paraformaldehyde
ThermoFisher Scientific
Used for fixing cells.
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Nd:YAG laser
Minilite II
Continuum Inc.
Desorption laser for NDPI-MS.
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Optical fiber
SFS50/125/250Y
Fiberguide Industries
Used for laser conduction and focusing in NDPI-MS.
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