A detection and analysis method of trace triptolide in a biological sample
A technology of triptolide and biological samples, which is applied in the field of detection and analysis of trace amounts of triptolide in biological samples, can solve the problems of low content, matrix interference, accuracy and mass spectrometry ionization efficiency, etc., and achieve the recovery rate High, reduce matrix interference, overcome the effect of long derivatization reaction time
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Embodiment 1
[0040] Chromatographic separation and mass spectrometry qualitative and quantitative analysis methods of triptolide:
[0041] In the range of 3-5000 pg / mL, prepare 7 different concentrations d 0 - MCR6G labeled triptolide standard solution (20 pg / mL, 400 pg / mL, 800 pg / mL, 1500 pg / mL, 2000 pg / mL, 3000 pg / mL, 4000pg / mL), where d 3 -MCR6G-labeled standard (2500 pg / mL) was used as fixed internal standard. The specific derivatization process is as follows: 1 part of the above-mentioned standard solution with different concentration levels, 25 μL CMPI (7 wt%) and 25 μL DMAP (10.5 wt%) acetonitrile solution, 150 μL d 0 -MCR6G or d 3 - MCR6G acetonitrile solution, add to a 1.5 mL centrifuge tube one by one, vortex for 10 seconds. Seal and react in a microwave reactor (840 W) at 56 °C for 6.5 min. 7 levels of concentration d 0 -MCR6G standard derivative and d 3 -MCR6G-labeled immobilized standard derivatives 1:1 respectively ( V / V ) to mix and shake well. The magnetic di...
Embodiment 2
[0046]The extraction of triptolide in the brain microdialysate comprises the following steps:
[0047] Take 200 μL of rat brain microdialysate into a centrifuge tube, blow dry with nitrogen, and redissolve the residue in 200 μL of acetonitrile for stable isotope labeling derivatization. Take 50 µL brain microdialysate acetonitrile reconstitution solution or standard solution, 25 µL CMPI (8 wt%) and 25 µL DMAP (15 wt%) acetonitrile solution, 150 µL d 0 -MCR6G or d 3 - MCR6G acetonitrile solution, add to a 1.5 mL centrifuge tube one by one, vortex for 10 seconds. Seal and react in a microwave reactor (850 W) at 60 °C for 6.5 min. d 0 -MCR6G-labeled brain microdialysate and d 3 -MCR6G labeled standard 1:1 ( V / V ) to mix and shake well. Disperse 10 mg of magnetic molecularly imprinted polymer into the above mixed solution and shake for 60 minutes. Magnetic separation, the adsorbed d 0 -MCR6G- triptolide derivative desorbed down. Magnetically separated and blown dry w...
Embodiment 3
[0049] The extraction of triptolide in the hemodialysate comprises the following steps:
[0050] Take 200 μL of rat blood microdialysate into a centrifuge tube, blow dry with nitrogen gas, and redissolve the residue in 200 μL of acetonitrile for stable isotope labeling derivatization. Take 50 µL hemodialysate acetonitrile reconstituted solution or standard solution, 25 µL CMPI (7 wt%) and 25 µL DMAP (14 wt%) acetonitrile solution, 100 µL d 0 -MCR6G or d 3 -MCR6G acetonitrile solution, add to 1.5mL centrifuge tube in turn, vortex for 10 seconds. Seal and react in a microwave reactor (820 W) at 57 °C for 6 min. d 0 -MCR6G-labeled hemodialysate and d 3 -MCR6G labeled standard 1:1 ( V / V ) to mix and shake well. Disperse 12 mg of magnetic molecularly imprinted polymer into the above mixed solution and shake for 60 minutes. Magnetic separation, the adsorbed d 0 -MCR6G- triptolide derivative desorbed down. Magnetically separated and blown dry with nitrogen. The residue...
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