Exosomes, their preparation method and their application in the preparation of drugs for the treatment of lung cancer
A technique of adding exosomes, which is applied in the field of biomedicine, can solve the problems that exosomes have not been seen and the anti-tumor activity has not been fully confirmed, so as to enhance the anti-lung tumor activity, enhance the cytotoxicity, and enhance the effect of effect
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Embodiment 1
[0060] The cultivation of embodiment 1CIK cell
[0061] 1. Cord blood mononuclear cell extraction:
[0062] Fresh umbilical cord blood was anticoagulated with heparin, and umbilical cord blood mononuclear cells (CBMNC) were separated by Ficoll-Hypaque method. Mix cord blood and phosphate buffer saline (PBS solution) in equal volumes, and slowly add it to Ficoll-Hypaque (purchased from GE) at a volume ratio of 1:1, centrifuge at 20°C, 400×g for 25 minutes; carefully draw The CBMNC band layer in the centrifuge tube was resuspended with PBS solution and centrifuged at 200×g for 15 minutes; the supernatant was removed, and the pellet was resuspended with PBS solution and centrifuged at 200×g for 15 minutes to obtain cord blood single nuclei cell.
[0063] 2. Cell culture:
[0064] According to different groups, the above-mentioned CBMNCs were resuspended and cultured. See Table 1 for the grouping situation, the addition amount of various components (ATP corresponds to the final...
Embodiment 2CI
[0080] Example 2Extraction and identification of CIK cell-derived exosomes
[0081] 1. Extraction of exosomes
[0082] Exosomes were extracted from the cell culture fluid obtained according to the grouping in Table 1, specifically:
[0083] Collect 20mL of the above cell culture supernatant, centrifuge at 2000×g for 30min, take the supernatant, discard cell debris and other precipitates; centrifuge at 4°C and 10000×g for 60min to obtain a concentrated solution containing exosomes; Centrifuge the concentrated solution at 4°C and 100,000×g for 60 minutes to collect the bottom precipitate; resuspend the obtained precipitate in PBS buffer, and centrifuge again at 100,000×g for 60 minutes to collect the bottom precipitate, which is CIK cell exosomes; The body was resuspended with 2ml of PBS buffer, sterilized by filtration with a 0.22μm filter membrane, and stored at -80°C.
[0084] 2. Identification of Exosomes
[0085] ① Morphological observation of exosomes:
[0086] The exo...
Embodiment 3
[0095] Example 3 Effect of KRN7000 and ATP on the expression of cytotoxic protein in exosomes of CIK cells
[0096] The levels of FasL and perforin in exosomes were detected by protein immunoassay:
[0097] Use RIPA lysate to lyse the exosomes in each group for 30 minutes, and use a homogenizer to homogenize the protein (15s×3 times); after standing for 30 minutes, centrifuge the above homogenate at 4°C and 12,000g for 15 minutes; For protein quantification with the BCA kit, adjust the total protein concentration to the same level; add 5× loading buffer and boil for 5 minutes; load the above solution, conduct shrink gel electrophoresis at 80V for about 30 minutes, and conduct separation gel electrophoresis at 120V About 60min; the protein was transferred to PVDF membrane by electrotransfer (250mA, 2h), and blocked with blocking solution for 1h at room temperature; After incubation overnight, the membrane was washed with TBST (10min×3 times); after that, it was incubated with ...
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