Literature DB >> 10698976

Efficiencies of translation in three reading frames of unusual non-ORF sequences isolated from phage display.

E Goldman1, M Korus, W Mandecki.   

Abstract

An unusual nucleotide sequence, called H10, was previously isolated by biopanning with a random peptide library on filamentous phage. The sequence encoded a peptide that bound to the growth hormone binding protein. Despite the fact that the H10 sequence can be expressed in Escherichia coli as a fusion to the gene III minor coat protein of the M13 phage, the sequence contained two TGA stop codons in the zero frame. Several mutant derivatives of the H10 sequence carried not only a stop codon, but also showed frameshifts, either +1 or -1 in individual isolates, between the H10 start and the gene III sequences. In this work, we have subcloned the H10 sequence and three of its derivatives (one requiring a +1 reading frameshift for expression, one requiring a -1 reading frameshift, and one open reading frame) in gene fusions to a reporter beta-galactosidase gene. These sequences have been cloned in all three reading frames relative to the reporter. The non-open reading frame constructs gave (surprisingly) high expression of the reporter (10-40% of control vector expression levels) in two out of the three frames. A site-directed mutant of the TGA stop codon (to TTA) in the +1 shifter greatly reduced the frameshift and gave expression primarily in the zero frame. By contrast, a site-directed mutant of the TGA in the -1 shifter had little effect on the pattern of expression, and alteration of the first TGA (of two) in H10 itself paradoxically reduced expression by half. We believe these phenomena to reflect a translational recoding mechanism in which ribosomes switch reading frames or read past stop codons upon encountering a signal encoded in the nucleotide sequence of the mRNA, because both the open reading frame derivative (which has six nucleotide changes from parental H10) and the site-directed mutant of the +1 shifter, primarily expressed the reporter only in the zero frame.

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Year:  2000        PMID: 10698976     DOI: 10.1096/fasebj.14.3.603

Source DB:  PubMed          Journal:  FASEB J        ISSN: 0892-6638            Impact factor:   5.191


  11 in total

1.  Genetic analysis of the basis of translation in the -1 frame of an unusual non-ORF sequence isolated from phage display.

Authors:  Jennifer Zemsky; Wlodek Mandecki; Emanuel Goldman
Journal:  Gene Expr       Date:  2002

Review 2.  Ribosomal frameshifting and transcriptional slippage: From genetic steganography and cryptography to adventitious use.

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4.  Identification of immunogenic proteins and generation of antibodies against Salmonella Typhimurium using phage display.

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7.  stg fimbrial operon from S. Typhi STH2370 contributes to association and cell disruption of epithelial and macrophage-like cells.

Authors:  Liliana Berrocal; Juan A Fuentes; A Nicole Trombert; Matías R Jofré; Nicolás A Villagra; Luis M Valenzuela; Guido C Mora
Journal:  Biol Res       Date:  2015-07-07       Impact factor: 5.612

8.  Mining gut microbiome oligopeptides by functional metaproteome display.

Authors:  Jonas Zantow; Sarah Just; Ilias Lagkouvardos; Sigrid Kisling; Stefan Dübel; Patricia Lepage; Thomas Clavel; Michael Hust
Journal:  Sci Rep       Date:  2016-10-05       Impact factor: 4.379

9.  High-Throughput Sequencing of Phage Display Libraries Reveals Parasitic Enrichment of Indel Mutants Caused by Amplification Bias.

Authors:  Sander Plessers; Vincent Van Deuren; Rob Lavigne; Johan Robben
Journal:  Int J Mol Sci       Date:  2021-05-24       Impact factor: 5.923

10.  Mimotopes and proteome analyses using human genomic and cDNA epitope phage display.

Authors:  Mullaney P B; Marks D J; Pallavicini G M
Journal:  Comp Funct Genomics       Date:  2002
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