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A streamlined method to obtain biologically active TcdA and TcdB toxins from Clostridioides difficile

Sapa, A. A. D.; Brosse, A.; Coullon, H.; Pean de Ponfilly, G.; Candela, T.; Le Monnier, A.

2023-07-19 microbiology
10.1101/2023.07.19.549664 bioRxiv
Show abstract

The major virulence factors of Clostridioides difficile (C. difficile) are enterotoxin A (TcdA) and cytotoxin B (TcdB). The study of toxins is a crucial step in exploring the virulence of this pathogen. Currently, the toxin purification process is either laborious and time-consuming in C. difficile or performed in heterologous hosts. Therefore, we propose a streamlined method to obtain functional toxins in C. difficile. Two C. difficile strains were generated each harboring a sequence encoding a His-tag at the 3 end of C. difficile 630{Delta}erm tcdA or tcdB genes. Each toxin gene is expressed using the Ptet promoter inducible by anhydro-tetracycline. The purification yields were estimated to be 0.28 mg per liter and 0.1 mg per liter for rTcdA and rTcdB, respectively. In this study, we successfully developed a simple routine method that allows the production and purification of biologically rTcdA and rTcdB active toxins with similar activities compared to native toxins.

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