The accurate detection of glucose is critical for clinical diagnostics and metabolic monitoring. This study focused
on the successful synthesis and incorporation of the glucose dehydrogenase (GDH) gene sequence from Bur�kholderia cepacia into a plasmid, followed by codon optimization and modification of cysteine motifs for
increased expression in E. coli. The engineered E. coli strain demonstrated efficient heterologous expression of
stable GDH. Remarkably, the recombinant strain not only enabled cost-effective GDH production but also
exhibited excellent glucose catalytic activity, with a detection range of 1 μM to 10 mM and a minimum detectable
concentration of 1 μM. This functionality makes it sui... More
The accurate detection of glucose is critical for clinical diagnostics and metabolic monitoring. This study focused
on the successful synthesis and incorporation of the glucose dehydrogenase (GDH) gene sequence from Bur�kholderia cepacia into a plasmid, followed by codon optimization and modification of cysteine motifs for
increased expression in E. coli. The engineered E. coli strain demonstrated efficient heterologous expression of
stable GDH. Remarkably, the recombinant strain not only enabled cost-effective GDH production but also
exhibited excellent glucose catalytic activity, with a detection range of 1 μM to 10 mM and a minimum detectable
concentration of 1 μM. This functionality makes it suitable for applications of AuNPs/SPE/glucose biosensors,
offering high sensitivity for glucose detection—a novel achievement not previously reported. These findings have
the potential to advance the clinical utilization of AuNPs/tetracysteine/GDH-modified biosensors and may
promote the development of GDH-based electrochemical biosensors.
