Publication protocol
"The yeast expression library vectors were linearized by SacI digestion and transformed into P . pastoris X-33 with the lithium chloride transformation method described in EasySelectTM Pichia expression kit user manual (Invitrogen). Transformants were initially grown on YPD plates supplemented with 100 µg/ml zeocin. After integration of the plasmid into the yeast genome was confirmed by colony PCR, resulting colonies were transferred to YPD plates with 200, 500 and 1000 µg/ml zeocin for determination of the copy number of integrants. The subsequent comparisons of secreted proteins were only made between transformants with approximately the same copy numbers as determined by the same concentration range of drug resistance against zeocin.
The experimental protocol from EasySelectTM Pichia expression kit user manual to express recombinant Pichia pastorish has been followed. Briefly, the selected colonies were initially cultivated (shaking vigorously at 250 rpm) in BMGY medium at 28-30°C until the value of OD600 reached 2 approximately. After centrifugation and removal of BMGY, cell pellets were re-suspended in BMMY to an OD600 of 1 to induce expression. The volume of the culture should be no more than 10-30% of the total well/tube/flask volume to ensure sufficient aeration. Methanol was added to a final concentration of 1% every 24 hours to maintain induction. Yeast culture media were sampled and assayed every 24 hours. Small-scale cultivation and expression using 96-deep-well plates (Bel-Art Scienceware, NJ, USA) were carried out as previously described [42,43] whenever high-throughput screening of the secretory productivity was needed."
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