Method for purifying gene-recombinant insulin precursor
A technology of insulin precursor and gene recombination, which is applied in the direction of insulin, chemical instruments and methods, peptide preparation methods, etc. It can solve the problems that the fractionation medium cannot be applied to large-scale production, the pigment cannot be completely removed, and it is unfavorable for large-scale production. , to achieve the effect of low cost, high speed, high purity and recovery rate
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[0022] 1. After passing the pretreated powdered activated carbon through a 60-mesh sieve, weigh 20 grams and add it to 2 liters of fermentation broth. Stir with a glass rod for 10 minutes, then centrifuge in a high-speed centrifuge at 8,000 rpm for 20 minutes, and collect 1 L of supernatant.
[0023] 2. Weigh 30 grams of pretreated granular activated carbon (20mm×40mm), and put it on a 20cm×2.6cm glass column. After washing with 1% acetic acid aqueous solution, the collected supernatant was introduced into the column with a pump, and the flow rate was controlled at 3 mL / min. After the sample was loaded, the sample was also ejected from the activated carbon column with 1% acetic acid aqueous solution. Collect 1.2 L of breakthrough solution.
[0024] 3 Cationic filler sp550EC, take 100mL and put it on a 20cm×2.6cm glass column.
[0025] The balance solution is pH4.0, 50mmolNaAc-HAC
[0026] The washing solution is pH4.0, 50mmolNaAc-HAC+0.1mol / L NaCl+40% ethanol
[0027] The...
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