Fluorescence immunoassay of E-coli using anti-lipopolysaccharide antibodies isolated from human serum

Authors
Bong, Ji-HongKim, JiyunLee, Ga-YeonPark, Jun-HeeKim, Tae-HunKang, Min-JungPyun, Jae-Chul
Issue Date
2019-02-01
Publisher
ELSEVIER ADVANCED TECHNOLOGY
Citation
BIOSENSORS & BIOELECTRONICS, v.126, pp.518 - 528
Abstract
In this work, the gram-negative bacterium Escherichia colt strain BL21(DE3) (with lipopolysaccharide (LPS) in its outer membrane) and its modified ClearColi (TM). strain (lacking LPS) were used for the separation of anti-LPS antibodies from human serum by the following steps: (1) binding of the serum proteins to BL21(DE3); (2) dissociation of the bound proteins (including anti-LPS antibodies) from BL21(DE3) with acid; (3) filtering of the dissociated proteins using ClearColi to remove unwanted proteins; and (4) separation of the antibody fraction by protein-A column chromatography. The binding properties of the separated antibodies were analyzed by fluorescence-activated cell sorting to confirm their selective binding to LPS on the outer membrane of BL21(DE3), and by thermophoretic immunoassay to estimate their dissociation constant. The in vitro applicability of the separated anti-LPS antibodies was demonstrated through a fluorescence assay of BL21(DE3), after immobilizing the antibodies onto a modified microplate surface. The electrochemical detection of BL21(DE3) was also achieved after immobilizing the anti-LPS antibodies onto a gold electrode.
Keywords
OUTER-MEMBRANE; E. COLI; INTERDIGITATED ELECTRODE; MASS-SPECTROMETRY; SPR BIOSENSOR; CELLS; IMMOBILIZATION; PURIFICATION; EXPRESSION; PARYLENE; OUTER-MEMBRANE; E. COLI; INTERDIGITATED ELECTRODE; MASS-SPECTROMETRY; SPR BIOSENSOR; CELLS; IMMOBILIZATION; PURIFICATION; EXPRESSION; PARYLENE; LPS; Anti-LPS antibody; Separation; Human serum; ClearColi
ISSN
0956-5663
URI
https://pubs.kist.re.kr/handle/201004/120365
DOI
10.1016/j.bios.2018.10.036
Appears in Collections:
KIST Article > 2019
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