development of phage-based single chain fv antibody reagents for detection of yersinia pestis发展phage-based单链阵线抗体试剂检测鼠疫杆菌.pdfVIP
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development of phage-based single chain fv antibody reagents for detection of yersinia pestis发展phage-based单链阵线抗体试剂检测鼠疫杆菌
Development of Phage-Based Single Chain Fv Antibody
Reagents for Detection of Yersinia pestis
Antonietta M. Lillo., Joanne E. Ayriss., Yulin Shou, Steven W. Graves, Andrew R. M. Bradbury*,
Peter Pavlik
Bioscience Division, Los Alamos National Laboratory, Los Alamos, New Mexico, United States of America
Abstract
Background: Most Yersinia pestis strains are known to express a capsule-like antigen, fraction 1 (F1). F1 is encoded by the
caf1 gene located on the large 100-kb pFra plasmid, which is found in Y. pestis but not in closely related species such as
Yersinia enterocolytica and Yersinia pseudotuberculosis. In order to find antibodies specifically binding to Y. pestis we
screened a large single chain Fv antibody fragment (scFv) phage display library using purified F1 antigen as a selection
target. Different forms of the selected antibodies were used to establish assays for recombinant F1 antigen and Y. pestis
detection.
Methods: Phage antibody panning was performed against F1 in an automated fashion using the Kingfisher magnetic bead
system. Selected scFvs were screened for F1-binding specificity by one-step alkaline phosphatase enzyme linked
immunosorbant assay (ELISA), and assayed for binding to recombinant antigen and/or Y. pestis by flow cytometry and
whole-cell ELISA.
Results: Seven of the eight selected scFvs were shown to specifically bind both recombinant F1 and a panel of F1-positive
Yersinia cells. The majority of the soluble scFvs were found to be difficult to purify, unstable and prone to cross-reactivity
with F1-negative Yersinia strains, whereas phage displayed scFvs were found to be easy to purify/label and remarkably
stable. Furthermore direct fluorescent labeling of phage displaying scFv allowed for an easy one-step flow cytometry assay.
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