Fig. 5

Purification of starch-binding enzymes from the secretome. β-cyclodextrin-sepharose affinity chromatography purification of the Aspergillus nidulans wheat starch culture supernatant harvested after 5 days (lane II). Three dominant bands were identified using mass spectrometry (MALDI-TOF MS, see “Methods” section). The bands were identified as glucoamylase (1), α-amylase (2 and 2*-CBM20 domain), and AnLPMO13A (3). Molecular mass marker in kDa (lane I)