@ARTICLE{Ebrahimi, author = {Rezaeiani, Siamak and Ebrahimi, Firoz and Honari, Hossein and Hajizade, Abbas and Barati, Babak and }, title = {CLONING AND EXPRESSION OF CLOSTRIDIUM BOTULINUM TYPE B BINDING DOMAIN E. COLI}, volume = {25}, number = {6}, abstract ={   Backgrounds & Aims: Botulism is caused by botulinum toxin. The best way to avoid the neurotoxin syndrome caused by BONT/B is to use recombinant vaccine made of BONT/B binding domain because binding domain has sufficient epitops to stimulate immune response. Materials & Methods: Initially BONT/B binding domain gene sequence were obtained from GenBank. Then the primers were designed. PCR reaction was performed. Then gene was ligated to pGEM-Teasy vactor. After verifying the transformation E.coli DH 5 α , subcloning was done. Pet28(a)+ vector was introduced to SDS-PAGE and Western blot confirmed production of the protein. Results: The results obtained from PCR sequencing via IPTG induction and expression analysis by SDS-PAGE and its confirmation by Western blot indicated the cloning and expression process accuracy. Conclusion: Finally, this method may be suitable for production of recombinant vaccines without any side effects. Cloning and expression of this vaccine candidate were conducted successfully and its immunization potential should be investigated.    SOURCE: URMIA MED J 2014: 25(6): 510 ISSN: 1027-3727 }, URL = {http://umj.umsu.ac.ir/article-1-2366-en.html}, eprint = {http://umj.umsu.ac.ir/article-1-2366-en.pdf}, journal = {Studies in Medical Sciences}, doi = {}, year = {2014} }