Part:BBa_K4879011

ScRAD52 Expression Construct

The transcriptional unit for ScRAD52, designed for expression in Y. lipolytica in order to increase homologous recombination probability to about 95%.

Characterization

Cloning: The construct, along with homologous flanking sequences corresponding to the faa1 gene locus, were synthesized by iGEM’s DNA synthesis partner IDT. The resulting gene fragment was then PCR amplified with the respective primers to attain a higher copy number of the fragment. The amplification of the fragment was verified by running a 0.8% agarose gel, with the fragments expected to show at around the 3000 bp region.

Fig 1: Lane 1 is the DNA ladder, with lanes 8-11 showing successful amplicons.

The amplified fragment was then gel-extracted and assembled together with the guaB expression construct with the help of the NEBuilder HiFi DNA Assembly kit, and subsequently transformed into our chassis.

Validation: The transformed yeast culture was then plated onto the selection plates containing about 1000-2000 µg/ml of mycophenolic acid and were incubated at 30°C. The growth of the yeast on the selection plates confirms the functional validity of the expression construct.

Fig 2: The growth of transformed Y. lipolytica on the MPA selection plate, confirming part functionality.

Sequence and Features