Recombinant production and affinity purification of the FraC pore forming toxin using hexa-His tag and pET expression cassette

Abstract:
Objective(s)
A newly-introduced protein toxin from a sea anemone, namely fragaceatoxin C is a protein with molecular weight of 20 kDa and pore-forming capability against cell membranes has recently grasped great attentions for its function. In this study, its coding sequence cloned as a fusion protein with His-tag for simple production and rapid purification.
Materials And Methods
After PCR amplification using NcoI and HindIII-harboring primers, the gene fragment was cloned into pET-28a(). Escherichia coli BL21 was used for expression of constructed vector and toxin expression was verified by SDS-PAGE. For one-step purification Ni-NTA sepharose affinity chromatography was employed. For examination of purified toxin function, RBC hemolytic test was conducted.
Results
The results showed that the FraC-coding gene was successfully cloned between NcoI and HindIII restriction sites and purified with affinity chromatography. Densitometric analysis represented the purity of approximately 97%. Hemolytic test indicated the purified FraC had remarkable lytic activity on RBC and almost lysed 50% of cells at the concentration value of 6.25 nM.
Conclusion
The results indicated that not only purified toxin preserved its activity during expression and purification processes but also exerted its function at lower concentrations so that even the 0.09 nM displayed hemolytic effect.
Language:
English
Published:
Iranian Journal of Basic Medical Sciences, Volume:20 Issue: 4, Apr 2017
Pages:
380 to 385
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