Pichia pastoris alcohol oxidase ZZA1 and ZZA2 regulatory regions for heterologous gene expression

Assignee

• Biosource Technologies, Inc. · US

Inventors

• Monto Kumagai · Davis, US
• Genadie G. Sverlow · Vacaville, US

Key dates

Classification

• Technology area (CPC Y)Emerging Cross-Sectional Technologies
• CPC primaryY02E50/10
• WIPO fieldBiotechnology
• WIPO sectorChemistry

Abstract

Two novel genomic clones, ZZA1 and ZZA2, were isolated which encode for Pichia pastoris alcohol oxidase isozymes. The 5' non-coding region of ZZA1 contains common structural features involved in the transcription and translation of eukaryotic genes. Comparison of the nucleotide sequences of the ZZA1 and AOX1 51 noncoding regions showed that they are 66% similar to each other. The rice .alpha.-amylase gene OS103 was placed under the transcriptional control of the ZZA1 promoter. The nucleotide sequences of ZZA1 and other methanol-regulated promoters were analyzed. A highly conserved sequence (TTGNNNGCTTCCAANNNNNTGGT) (SEQ ID NO:2) was found in the 51 flanking region. A yeast strain containing the ZZA1 -OS103 fusion and secreting biologically active a-amylase into the culture media while converting starch to ethanol was produced. The ZZA1 and ZZA2 regulatory sequences may be used to contol the expression of other heterologous proteins in multiple yeast species. Methods of purifying proteins that are regulators of alcohol oxidase expression (referred to as AOER proteins) and methods of isolating these proteins are also provided. The invention also provides for the efficient conversion …