Novel cold-adapted raw-starch digesting α-amylases from Eisenia fetida: Gene cloning, expression, and characterization

Kana Tsukamoto; Shingo Ariki; Masami Nakazawa; Tatsuji Sakamoto; Mitsuhiro Ueda

doi:10.1016/j.btre.2021.e00662

Novel cold-adapted raw-starch digesting α-amylases from Eisenia fetida: Gene cloning, expression, and characterization

Biotechnol Rep (Amst). 2021 Aug 17:31:e00662. doi: 10.1016/j.btre.2021.e00662. eCollection 2021 Sep.

Authors

Kana Tsukamoto¹, Shingo Ariki¹, Masami Nakazawa¹, Tatsuji Sakamoto¹, Mitsuhiro Ueda¹

Affiliation

¹ Graduate School of Life and Environmental Sciences, Osaka Prefecture University, Osaka, 599-8531, Japan.

Abstract

We identified the raw-starch-digesting α-amylase genes a earthworm Eisenia fetid α amylase I and II (Ef-Amy I and Ef-Amy II). Each gene consists of 1,530 base pairs (bp) that encode proteins of 510 amino acids, as indicated by the corresponding mRNA sequences. Ef-Amy I and II showed an 89% amino acid identity. The amino acid sequences of Ef-Amy I and II were similar to those of the α-amylases from porcine pancreas, human pancreas, Tenebrio molitor, Oryctolagus cuniculus, and Xenopus (Silurana) tropicalis. Each gene encoding mature Ef-Amy I and II was expressed in the GS115 strain of Pichia pastoris. The molecular masses of the recombinant Ef-Amy I and II were 57 kDa each, and catalytically important residues of α-amylases of the GH family 13 were conserved in both proteins. These amylases exhibited raw-starch-digesting activity at 4 °C. The substrate specificities of rEf-Amy I and II were dissimilar. rEf-Amy I and II were shown to be active even in 40% ethanol, 4 M NaCl, and 4 M KCl.

Keywords: Cold-adapted enzyme; Eisenia fetida; Glycoside hydrolase family 13; Raw-starch-digesting enzyme; Αlpha-amylase.