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Nature-inspired engineering of an F-type lectin for increased binding strength

Glycobiology. 2018; 
Mahajan S, Ramya TNC
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Codon Optimization 1) was codon-optimized, custom-synthesized (Genscript), and cloned in pUC57, and the sequence corresponding to the FLD (referred to as SrFLD) amplified by PCR with appropriate primers (forward primer, 5’-CATGCCATGGCGCGTCCGAATCTGAGTCTGGG-3’, and reverse primer, 5’-GCAGAAGTCCAAGTGCGTGGCCTCGAGCGG-3’) and subcloned in the expression vector, pET-28a(+) within NcoI and XhoI sites to create SrFLD-pET-28a(+) such that the plasmid would encode recombinant SrFLD with a C-terminal hexahistidine tag....1), was codon optimized and synthesized from Genscript, Piscataway, NJ in pUC57 and sub-cloned in the expression vector, pET-28a(+) within Nco I and Xho I sites to create BfDupFLD-pET-28a(+) such that the plasmid would encode recombinant BfDupFLD with a C- terminal hexahistidine tag. Get A Quote

摘要

Individual lectin-carbohydrate interactions are usually of low affinity. However, high avidity is frequently attained by the multivalent presentation of glycans on biological surfaces coupled with the occurrence of high order lectin oligomers or tandem repeats of lectin domains in the polypeptide. F-type lectins are l-fucose binding lectins with a typical sequence motif, HX(26)RXDX(4)R/K, whose residues participate in l-fucose binding. We previously reported the presence of a few eukaryotic F-type lectin domains with partial sequence duplication that results in the presence of two l-fucose-binding sequence motifs. We hypothesized that such partial sequence duplication would result in greater avidity of lectin-l... More

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