Validation of the Three Binding Heads

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Cellulose Binding

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We designed a fusion protein between the Carbohydrate Binding Module type 3a and a fluorescent reporter and named it Sirius as a reference to the brightest star of the norther hemisphere. Its purpose is to validate the association of our system towards cellulose. We demonstrated, using mRFP1 alone as negative control, the binding of our protein as showned in figure 2. We were then confident in the binding of our protein to cellulose.

Biotinylated compound affinity

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Our second construction consisted on our protein Cerberus but lacking the un natural amino acid. This construction aimed to prove the binding affinity of our system toward biotinylated compounds. As biotinylation can be both performed at high yield in vivo and in vitro, this construction is already a molecular binding plateform, allowing the purification of biotinylated compounds at low cost, using cellulose. We validated this construction using biotinylated mTag Blue Fluorescent Protein (figure3.a), biotinylated in vivo in E. coli and Scygonadin, an anti microbial peptide, produced in Pichia pastoris (figure 3.b).

Click chemistry

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Our plateform aims to have a binding capacity as wide as possible. The azide groupment offer a high efficiency covalent bound formation through cycloadditionreaction, mostyl known by Click chemistry. The possibilities offered by this system are therefore included in the unnatural amino acid : 4-azido-L-phenylalanine. We designed our protein to bear an Amber stop codon for unnatural amino acid integration in our plateform. We confirmed the activity of this integration using DBCO-Fluorescein as showed in figure 4. We also functionnalized cellulose using paramagnetic beads (see video below) which shows the broad range functionnalization possibilities that our system offers.