研究目的
To study the effect of drying technique and surface pre-treatment on the cytotoxicity and dissolution rate of luminescent porous silicon quantum dots in model fluids and living cells.
研究成果
The drying process and surface pre-treatment significantly affect the dissolution rate of luminescent silicon QDs in model fluids and living cells. SCD-Si QDs showed faster dissolution and lower apparent cytotoxicity compared to AD-Si QDs, which is important for their use in theranostics combining drug delivery and luminescent imaging.
研究不足
The study is limited to in-vitro conditions and does not explore in-vivo biodegradation and toxicity profiles. The impact of local environmental variations on degradation time is not fully addressed.
1:Experimental Design and Method Selection
The study used a combination of photoluminescence and Raman micro-spectroscopy to investigate the dissolution rate of Si QDs in model liquids and living cells. Porous silicon particles were obtained by mechanical milling of electrochemically etched mesoporous silicon films.
2:Sample Selection and Data Sources
Porous silicon particles were subjected to super-critical drying with CO2 solvent (SCD) or air drying (AD) and then annealed at 600 C for 16 hours in 1% oxygen to achieve the nano-sized Si QDs.
3:List of Experimental Equipment and Materials
Transmission electron microscopy (TEM, LEO912 AB OMEGA), Malvern Instruments Mastersizer 2000, Micromeritics Tristar 3000, Fourier-transform infrared (FTIR) spectrometer (Bruker IFS 66v/S), Confotec? MR350 confocal Raman microscope.
4:Experimental Procedures and Operational Workflow
The samples were characterized by TEM, nitrogen gas adsorption/desorption analysis, FTIR spectroscopy, and Raman microspectroscopy. The dissolution of nanocrystals was evaluated by their PL quenching and changes in the Raman signal.
5:Data Analysis Methods
The sizes of the crystalline silicon core were calculated from the Raman scattering spectra. The dissolution rate was evaluated by changes in PL and Raman spectra.
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