Studying on expression and identification of human insulin in E. coli

Abstract

Insulin is a hormone that produced by beta cells inthe pancreas and regulated the glucose blood levels. Briefly, our strategy for the gene construction and expresion is described as follow. pET14bInsA vector contained gene A that encoding for the A peptide chain and pET14bInsB vector contained gene B that encoding for the B peptide chain. These vectors and the expression pET-32c(+) vector were digested by  NcoI and  BamHI. The released insulin A/B fragment and the opened plasmid pET-32c(+) were purified and ligated by T4 DNA ligase at 22^oC, overnight. The resulting recombinant plasmid pET32cInsA/B was transformed into the  E. coliBL21(DE3) strain. The expression of the fusion protein was observed by induction with 1 mM IPTG and analysed  by  SDS-PAGE. Two  new  protein  bands  with  the  size  of  aproximately  22  kDa (equvalent the size equvalent the size of fusion A) and 23 kDa (the size of fusion B) were then excised and  digested  with  trypsin  overnight. The  results  of  identifying  by  NanoLC-MS/MS (Nano  Liquid Chromatography - Tandem Mass Spectrometry) showed  that  the  recombinant protein  was  truely  the  fusion  A(B)-Trx  that  contained  different  peptides  from  chain  A/B  and thioredoxin. This result is an evidence to confirm  the successful construction and expression of chain A/B of insulin in the fusion form in E. coliwith pET-32c(+) vector.