ハイスループットシーケンシングを利用し全体プロテイン飽和突然変異誘発ライブラリの機能評価のためのプロトコル

0:43

Synthesis of NNS Sub-libraries for Each Amino Acid Position by Two-step PCR Site-directed Mutagenesis

1:53

Cloning of NNS Sub-libraries into Selection Vectors

3:47

Selection of the TEM-1 Whole-Protein Saturation Mutagenesis Library for Antibiotic Resistance

5:51

High Throughput Sequencing to Determine Fitness Effects of Mutations

8:44

Results: High Throughput Sequencing from Whole-Protein Saturation Mutagenesis

10:16

Conclusion