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Direct expression in E.coli of a functionally active protein A-snake toxin fusion protein
Authors:Ducancel, FrEdEric   Boulain, Jean-Claude   TrEmeau, Odile   MEnez, AndrE
Affiliation:Service de Biochimie, DÉpartement de Biologie, Laboratoire d'Ingenierie des ProtÉines, C.E.N. Saclay, 91191 Gif/Yvette, France.
Abstract:We constructed a recombinant expression plasmid encoding a proteinA–neurotoxin fusion protein. The fused toxin is directlyexpressed in the periplasmic space of Escherichia coli and canbe purified in the milligram range by a single immuno-affinitystep. The LD50 values of the fused toxin and native toxin are130 and 20 nmol/kg mouse respectively. The Kd values characterizingtheir binding to the nicotinic acetylcholine receptor (AcChoR)are respectively 4.8 ± 0.8 and 0.07 ± 0.03 nM.In contrast, the fused and native toxins are equally well recognizedby a toxin-specific monoclonal antibody which recognizes theAcChoR binding site. The lower toxicity of the fused toxin mightresult, therefore, from a steric hindrance, due to the presenceof the bulky protein A moiety (mol. wt = 31 kd) rather thanto a direct alteration of the ‘toxic’ site. Thefused toxin is more immunogenic than native toxin, since 1 nmolof hybrid toxin and 14 nmol of native toxin give rise to comparabletiters of antitoxin antibodies which, furthermore, are equallypotent at neutralizing neurotoxicity. The work described inthis paper shows that the use of fused toxins may be of paramountimportance for future development of serotherapy against envenomationby snake bites.
Keywords:expression/  fusion protein/  snake toxins
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