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Generation and Validation of a Shewanella oneidensis MR-1 Clone Set for Protein Expression and Phage Display
Author(s) -
Haichun Gao,
Donna Pattison,
Tingfen Yan,
Dawn M. Klingeman,
Xiaohu Wang,
Joseph F. Petrosino,
Lisa Hemphill,
XiuFeng Wan,
Adam B. Leaphart,
George M. Weinstock,
Timothy Palzkill,
Jizhong Zhou
Publication year - 2008
Publication title -
plos one
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.99
H-Index - 332
ISSN - 1932-6203
DOI - 10.1371/journal.pone.0002983
Subject(s) - shewanella oneidensis , orfs , biology , clone (java method) , biopanning , plasmid , computational biology , microbiology and biotechnology , phage display , genome , genomic library , library , genetics , gene , open reading frame , peptide library , peptide sequence , bacteria , antibody , 16s ribosomal rna
A comprehensive gene collection for S. oneidensis was constructed using the lambda recombinase (Gateway) cloning system. A total of 3584 individual ORFs (85%) have been successfully cloned into the entry plasmids. To validate the use of the clone set, three sets of ORFs were examined within three different destination vectors constructed in this study. Success rates for heterologous protein expression of S. oneidensis His- or His/GST- tagged proteins in E. coli were approximately 70%. The ArcA and NarP transcription factor proteins were tested in an in vitro binding assay to demonstrate that functional proteins can be successfully produced using the clone set. Further functional validation of the clone set was obtained from phage display experiments in which a phage encoding thioredoxin was successfully isolated from a pool of 80 different clones after three rounds of biopanning using immobilized anti-thioredoxin antibody as a target. This clone set complements existing genomic ( e.g. , whole-genome microarray) and other proteomic tools ( e.g. , mass spectrometry-based proteomic analysis), and facilitates a wide variety of integrated studies, including protein expression, purification, and functional analyses of proteins both in vivo and in vitro .

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