Injectable hydrogels incorporating igf-1c polypeptides
A technology of IGF-1C and CS-IGF-1C, applied in the field of preparation of active injectable chitosan hydrogel
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Embodiment 1
[0099] Example 1: IGF-1C modified chitosan (CS) to obtain preparation of CS-IGF-1C
[0100] Solid Phase Synthesis of IGF-1C Polypeptide
[0101] The IGF-1C polypeptide was synthesized by a well-established solid-phase synthesis (SPPS) procedure using 2-chlorotrityl chloride resin and an amino acid whose side chain was protected by a tert-buty group and the amino group was protected by Fmoc. The steps are:
[0102] 1. The C-terminus of the first amino acid is grafted on the resin, and the loading rate is 0.6 mmol / g. 20% piperidine in N,N'-dimethylformamide (DMF) was used to remove the Fmoc protecting group of the amino group;
[0103] 2. Under the combined action of the condensing agent BTU and the catalyst DIPEA, the carboxyl group of the next amino acid combines with the free amino group; repeating the above steps, the polypeptide chain will continue to grow;
[0104] 3. The synthesis of hexanoic acid azide: ethyl 6-bromohexanoate and sodium azide are reacted in DMF, and t...
Embodiment 2
[0124] Example 2: Preparation and performance evaluation of CS-IGF-1C hydrogel
[0125] Preparation of CS-IGF-1C Hydrogel
[0126] (1) Dissolve CS-IGF-1C (1.5%, w / v) with acetic acid (0.1 mol / L), overnight at room temperature;
[0127] (2) Use distilled water to dialyze the CS solution against a dialysis membrane (molecular weight cut-off of 8 kDa–10 kDa) for 1 week to remove residual acetic acid;
[0128] (3) obtain CS-IGF-1C hydrochloride by freeze-drying;
[0129] (4) β-GP solution (2.29 mol / L) in ice bath was added dropwise to CS solution, and stirred for 0.5 hour under ice bath condition;
[0130] (5) The mixed solution is transferred to a 37°C incubator, and gelation can be seen in 5 minutes;
[0131] (6) The final concentration of β-GP in the mixed solution was 0.023 mol / liter, and the pH value of the CS-IGF-1C / β-GP solution after dialysis was 7.2.
[0132] Scanning electron microscopy to observe the morphology of hydrogels
[0133] After the hydrogels were freeze-...
Embodiment 3
[0140] Example 3: Biocompatibility of CS-IGF-1C
[0141] CCK-8 staining
[0142] We spread the material or hydrogel in a 96-well plate (5 μl / well) and placed the plate in an incubator (37°C) for 30 minutes (then used directly or stored at 4°C). On the one hand, in order to evaluate the effect of different concentrations of CS-IGF-1C material on cell viability, the material was coated on the well plate according to the gradient of 1%, 1.5%, 3%, 5% and 10% to culture ADSCs, and the culture was carried out after 24 hours. CCK-8 staining. On the other hand, in order to compare the effects of CS-IGF-1C and CS hydrogels on cell proliferation, the two hydrogels (at a concentration of 3%) were coated on well plates to culture ADSCs, and CCK-8 staining was performed 24 hours later. . Cells were plated at a concentration of 3×104 / well (4 wells / group). The specific dyeing method is as follows:
[0143] 1. Prepare CCK-8 staining solution (diluted according to CCK-8 stock solution:com...
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