Abstract
Site-directed mutagenesis of the glucansucrase gtf180 gene from Lactobacillus reuteri strain 180 was used to transform the active site region. The α-d-glucan (mEPS-PNNS) produced by the triple mutant V1027P:S1137N:A1139S differed in structure from that of the wild-type α-d-glucan (EPS180). Besides (α1→3) and (α1→6) linkages, as present in EPS180, mEPS-PNNS also
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