Part:BBa_K1023005

eforRed

Aspergillus niger codon-optimized (CO) eforRed chromoprotein encoding gene. We transformed Aspergillus niger with this construct after adding a mitochondrial signal sequence in order to show targeted organell colourization. Finally, on the day of the wiki-freeze, we observed the red mycelium (Fig.1)!

Fig.1 Transformant (left) A. niger shows clearly red mycelium compared to control (non codon-optimized eforRed

We performed PCR on our construct in fungal DNA and on our construct in the biobrick backbone as a positive control (Fig.2). The PCR showed faint bands for amplification of the transformant fungal DNA, while the bands for the positive controls were much more intense. The reason for this discrepancy might be that the (biobricking) primers we used fully anneal to the positive controls, while it only anneals partly to the eforRed sequence in the fungal DNA.

Fig.2 PCR of transformant A. niger; Lane 1 = marker, lane 2+3 = transformant fungal DNA, lane 5 = negative control, lane 7+8 = positive control (biobrick)

Usage and Biology

Chromoproteins have visible, intrinsic colours which are visible to the naked eye. This feature, as well as their small gene size, makes them feasible reporter molecules, i.e. as elective markers in co-transformations.

We codon-optimized (see design) this eforRed chromoprotein for usage in Aspergillus niger, thus trying to expand the usage of chromoproteins from prokaryotes to eukaryotes. So far we've observed red colour intensity in the fungal colonies.

We also tested the usability of our synthetic eforRed construct in E. coli. Results for this have not yet been obtained.

Sequence and Features