PCR and cloning of the lcs chimeric gene in
pcDNA3.1 vector and its expression in the cell line
Sepideh Saroughi1 , Maryam Zare2 , Rouhollah Kazemi3 ,
Mohammad-Javad Motamedi3 , Jafar Amani4
1- Department of Genetics, Payam Noor University, Tehran, Iran.
2- Department of Biology, Payam Noor University , Tehran, Iran.
3- Green Gene Company, Tehran, Iran
4- Chemical Injuries Research Center, Baqiyatallah University of Medical Sciences, Tehran, Iran
Abstract
Aim and Background: Diarrhea is the second most common cause of under-5 mortality. The most important strains of
Entrotoxigenic Escherichia coli causing Lt and St toxin cause diarrhea and
Entrohemoragic E.coli causing Shiga-like toxin secretion. Chlorine enterotoxin B subunit (Ctx) plays a key role in the development of diarrhea in Vibrio cholerae. More specific antibodies could be developed to counter these toxins by combining the CtxB, LtB and StB (LSC) epitopes and the production of trivalent vaccine. The aim of this study was to cloning
lsc gene into pcDNA3.1 to design a vaccine DNA.
Materials and Methods: The
lsc gene sequence was transferred to pcDNA3.1(+) vector after primer design and amplification by PCR. The pcDNA3.1(+) vector and the PCR product were digested using
HindIII and
EcoRI enzymes. Cloning of
lsc gene was performed in pcDNA3.1(+) vector and PCR. The clones were digested enzymatically. To ensure expression of lsc gene, it was transferred to HEK-293T cell and confirmed by Western blotting.
Results: The
lsc gene was confirmed by PCR and cloning in pcDNA3.1(+) vector using enzymatic digestion and a fragment length of 933 bp was detected and confirmed. Transfection kit was then transferred to HEK-293T cell and expression of the recombinant protein was confirmed by Western blotting and the protein was 39 kDa.
Conclusion: The results of the chimeric gene are well expressed in the cell line and confirmed by Western blotting that can be a good candidate for the fight against bacterial infection.
Keywords: Cloning,
lsc gene, DNA vaccine,
IAU science