Porous magnetic diagnosis and treatment agent, preparation method and use
A technology of photosensitizer and ferric tetroxide, which is applied in the field of biomedicine to achieve the effect of high-efficiency loading
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Embodiment 1
[0060] (1) Preparation of ferric oxide nanoparticles: The division weighs 300 mmoL of ferrous sulfate and 300 mmoL of ferric citrate and dissolves it in 100 mL of deionized water to prepare a solution, and stirs at 400 rpm to mix the solution completely; then add 500 mmoL of ascorbic acid, And add 0.3M sodium hydroxide to adjust the pH value of the solution to 9, after mixing and stirring again at 400rpm for 30min; transfer the solution to a hydrothermal reactor, react at 200 ° C for 5h, use a dialysis bag for dialysis, set Store in a refrigerator at 4° C. to obtain a dispersion suspension of ferric oxide nanoparticles. The dispersion suspension of the ferric oxide nanoparticles is adapted to a centrifuge for high-speed centrifugation, and the centrifuged product is dried to obtain the ferric oxide nanoparticles.
[0061] (2) Loading photosensitizer drug: Take 10 mL of the dispersion suspension of ferric oxide nanoparticles prepared above and uniformly mix with 10 mL of photos...
Embodiment 2
[0066] For in vitro tumor synergistic treatment, a mixture of physiological saline and diagnostic and therapeutic agent (the solvent is physiological saline, and the concentration of the diagnostic and therapeutic agent is 5 mg / mL) is placed in two 24-well cell culture plates, and sterilized for 2 hours. The PC3 cells were plated at 5 x 10 4 Cells / well were seeded into 24-well cell culture plates and cultured overnight. Then, cells in the first and second plates were irradiated with an 808 nm (NIR I biowindow) laser for 5 minutes, respectively. CCK-8 studies the metabolic activity of PC3 cells before and after laser irradiation. The absorbance of CCK-8 after 1 hour incubation with cells was read at 450 nm using a microplate reader (MK3, Thermo, USA).
[0067] test results image 3 As shown, there is no significant difference in the cell viability in the mixture of physiological saline and the diagnosis and treatment agent without laser excitation, indicating that the diagno...
Embodiment 3
[0070] will be about 10 7 PC3 cells were injected subcutaneously into the back of nude mice and fed for a period of time until the tumor volume reached 200 m 3 . The nude mice were divided into two groups, one group was injected with physiological saline, and the other group was injected with a diagnosis and treatment agent (the solvent was physiological saline, the concentration of the diagnosis and treatment agent was 5 mg / mL), and the physiological saline and the diagnosis and treatment agent were injected every 5 days, respectively. Then use 808nm (NIR Ibiowindow) laser to irradiate the tumor site, use FLIR TM The E60 camera records thermal images and temperatures of laser-irradiated mice. Nude mice were fed for 25 days to form tumor lumps, then, the tumor lumps were excised, and the tumor treatment effect was evaluated by measuring the volume and appearance of the tumor.
[0071] result Figure 4 and Figure 5 As shown, after injecting the diagnostic agent, the magn...
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