Expression of synthetic genes coding for completely new, nutritionally rich, artificial proteins |
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Authors: | Biernat, Jacek Koster, Hubert |
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Affiliation: | BIOSYNTECH Biochemische Synthesetechnik GmbH Stresemannstrasse 262-280, D-2000 Hamburg 50 1Institute für Organische Chemie und Biochemie Martin-Luther-King-Platz 6, D-2000 Hamburg 13, FRG |
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Abstract: | Synthetic genes (A, AB and AHB) constructed and cloned intopKK233-2 vector were recloned from the parent plasmid into thenew procaryotic expression vectors pGFY221N and pBIO52. GeneAFB (coding for all amino acids besides phenylalanine)was obtained by cassette mutagenesis from geneAB. The plasmid pGFY221N was constructed from pGFY218L by replacingthe PstI by an NcoI site; plasmid pBIO52 was derived from pGFY221Nthrough replacing the 221-bp EoRl/NcoI fragment with a syntheticDNA segment of 52 bp representing the Escherichia coli atpEgene translational initiation region. The genes A, AB, AHB andAFB in the vector pGFY221N were expressed with a six-amino-acid-longleader sequence; in pBIO52 the genes were expressed directly.in vitro expression experiments were successful with all thegenes except with the AHB gene integrated into pGFY221N. Inthe E. coli minicell system expression was demonstrated withthe A gene in pGFY221N and the AFB and AHB genes in pBIO52.Complete translation of the expressed genes AB, AFB andAHB in either the in vitro or in vivo systems could be shownby using 35S-labelled N-terminal methionine and C-terminal cysteine.Both amino acids occur only once in the peptide sequences. |
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Keywords: | artificial proteins/ cassette mutagenesis/ E. coli expression vectors/ protein engineering/ protein expression in vitro and in minicells |
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