Part:BBa_K2927051

pHMT-LbCas12a plasmid (LbCas12a protein purification)

T7 promoter can produce high yields in the transcription of E. coli when T7 RNA polymerase is present. The sequence we designed is for Cas12a protein expression and purification. Therefore, E.coli BL21 was used for producing our Cas12a protein. 10 times histidine and MBP are used for protein purification, and the TEV cutting site lets Cas12a protein separate from the composition (10X His-MBP-TEV site-Cas12a). 10 times histidine has a strong affinity with nickel ion, and the nickel ion is bind with nickel column. Therefore, we can separate the composition from the solution by nickel ion after breaking bacteria. In the second step of protein purification, the TEV enzyme cut the TEV cutting site for separate Cas12a protein from the composition. Next, we will get Cas12a protein from solution after gathering 10X His- MBP on nickel column.

Sequence and Features