Use of Aspergillus niger β-glucosidase II gene (bglII) promoter elements to construct an efficient expression vector.

Highlights: [•] Encoding of the novel promoter region of Aspergillus niger bglII was performed. [•] A high efficacy promoter d3 was constructed. [•] The transformant d3 was free from glucose repression. [•] The promoter of d3 transformant produced heterologous/homologous proteins in fungi. [ABSTRACT FROM AUTHOR]