Part:BBa_K1813004

CYP6G1

CYP6G1

Sequence and Features

Background of CYP6G1

As an enzyme capable of hydroxylating the 4 and 5 carbons of imidacloprid, it is capable of bestowing a significant protective effect to insects harboring this gene. It has an affinity to 6OH imidacloprid, allowing it to gnerate 4,5 OH imidacloprid [1], which has an ld50 of over 1 microgram vs 57 nanograms for imidacloprid [2]. Used in conjunction with CYP6CM1vQ, (BBa_K1813003) it can be extremely effective in bestowing imidacloprid resistance to an organism.
This coding sequence was synthesized and is codon optimized for E. coli. It was originally identified in Drosophila melanogaster, the common fruitfly [1]. This part is also used in BBa_K1613003 and BBa_K1813012

References

[1] Joußen, Nicole, et al. "Metabolism of imidacloprid and DDT by P450 CYP6G1 expressed in cell cultures of Nicotiana tabacum suggests detoxification of these insecticides in Cyp6g1‐overexpressing strains of Drosophila melanogaster, leading to resistance." Pest management science 64.1 (2008): 65-73.

[2]Suchail, S., Guez, D., & Belzunces, L. P. (2001). Discrepancy between acute and chronic toxicity induced by imidacloprid and its metabolites in Apis mellifera. Environmental toxicology and chemistry, 20(11), 2482-2486.