Part:BBa_M36014:Design

Glycogen Synthesis Actuator (alt2)

Design Notes

Composite of genomic sequences (glgC and glgA) coding for proteins involved in e. coli glycogen biosynthesis. Using different RBSs so that secondary structures and self pairing don't occur. Since there are only two genes, strong 5'UTRs were available for both. Based on the literature, we predict this part would result in a lesser increase in glycogen production than either part BBa_M36012 or BBa_M36014 because the effect of over expressing glgA seems to have lesser influence than glgS. glgC coding sequence was retained in all three designs because the mutant used here resulted in increased glycogen production even with normal expression levels.

References

Buschiazzo A, et al. Crystal structure of glycogen synthase: Homologous enzymes catalyze glycogen synthesis and degradation. EMBO J. 2004;23(16):3196–3205.

Dedhia NN, Hottiger T, Bailey JE. 1994. Overproduction of glycogen in Escherichia coli blocked in the acetate pathway improves cell growth. Biotechnol Bioeng 44(1):132–139

Kumar, A., Ghosh, P., Lee, Y.M., Hill, M.A. and Preiss, J. (1989) Biosynthesis of bacterial glycogen: determination of the amino acid changes that alter the regulatory properties of a mutant E. coli ADP-glucose synthase. J. Biol. Chem. 264, 10 464–10 471.

Meyer CR, Ghosh P, Remy E, Preiss J. Cloning, expression, and nucleotide sequence of a mutant glgC gene from Escherichia coli B. J Bacteriol. 1992 Jul;174(13):4509–4512

Preiss J ADPglucose pyrophosphorylase: basic science and applications in biotechnology. Biotechnol Annu Rev. 1996; 2: 259–279.

Preiss J., Shen L., Greenberg E., Gentner N. Biosynthesis of bacterial glycogen. IV. Activation and inhibition of the adenosine diphosphate glucose pyrophosphorylase of Escherichia coli. Biochemistry. 1966;5:1833–45.