Manipulation and expression of the maize zein storage proteins in Escherichia coli

• Published in: Journal of biotechnology Vol. 2; no. 3; pp. 157 - 175
• Main Authors: Norrander, Jan M., Vieira, Jeffrey, Rubenstein, Irwin, Messing, Joachim
• Format: Journal Article
• Language: English
• Published: Lausanne Elsevier B.V 01.01.1985; Amsterdam Elsevier; New York, NY
• Subjects: Agronomy; Biological and medical sciences; Biotechnology; cloning; Fundamental and applied biological sciences. Psychology; gene expression; genes; Industrial applications and implications. Economical aspects; M13mp and pUC vectors; oligonucleotide-directed in vitro mutagenesis; protein engineering; transfection; Zea mays; zein; protein engineering; oligonucleotide-directed in vitro mutagenesis; M13mp and pUC vectors; Monocotyledones; Bactériophage M13; Storage protein; Vegetals; Zea mays; Escherichia coli; Gene expression; Plasmid; Complementary DNA; Gramineae; Angiospermae; Bacteria; Spermatophyta; Zein; Escherichieae; Vector; Hybrid gene; Enterobacteriaceae
• ISSN: 0168-1656; 1873-4863
• DOI: 10.1016/0168-1656(85)90036-7

The cDNA sequence for the mature form of the zein protein A20 was inserted into the lac cloning region of two different M13mp phage vectors. Translation of these recombinant phage in E. coli cells produced a β-galactosidase—zein fusion protein. Another zein clone was constructed in which the entire coding sequence, including that of the signal peptide, was cloned into a M13mp vector. This clone was designed to produce a pre-zein protein which did not contain any β-galactosidase amino acids. Expression of these phage-coded proteins in E. coli cells was detected on Western blots using zein antibodies. Expression of the β-galactosidase—zein fusion protein was extremely low, comprising less than 1% of the total E. coli proteins. Levels of expression were increased slightly when this same sequence was cloned into a pUC-derived expression plasmid containing the highly efficient trp—lac promoter.