High Sensitivity Detection of Active Botulinum Neurotoxin by Glyco-Quantitative Polymerase Chain-Reaction
Author(s) -
SeokJoon Kwon,
Eun Ji Jeong,
Yung Choon Yoo,
Chao Cai,
GiHyeok Yang,
Jae Chul Lee,
Jonathan S. Dordick,
Robert J. Linhardt,
Kyung Bok Lee
Publication year - 2014
Publication title -
analytical chemistry
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.117
H-Index - 332
eISSN - 1520-6882
pISSN - 0003-2700
DOI - 10.1021/ac500262d
Subject(s) - chemistry , botulism , clostridium botulinum , botulinum neurotoxin , endopeptidase , toxin , polymerase chain reaction , neurotoxin , polymerase , dehalococcoides , dna , clostridiaceae , enzyme , microbiology and biotechnology , biochemistry , gene , biology , organic chemistry , vinyl chloride , copolymer , polymer
The sensitive detection of highly toxic botulinum neurotoxin (BoNT) from Clostridium botulinum is of critical importance because it causes human illnesses if foodborne or introduced in wounds and as an iatrogenic substance. Moreover, it has been recently considered a possible biological warfare agent. Over the past decade, significant progress has been made in BoNT detection technologies, including mouse lethality assays, enzyme-linked immunosorbent assays, and endopeptidase assays and by mass spectrometry. Critical assay requirements, including rapid assay, active toxin detection, sensitive and accurate detection, still remain challenging. Here, we present a novel method to detect active BoNTs using a Glyco-quantitative polymerase chain-reaction (qPCR) approach. Sialyllactose, which interacts with the binding-domain of BoNTs, is incorporated into a sialyllactose-DNA conjugate as a binding-probe for active BoNT and recovered through BoNT-immunoprecipitation. Glyco-qPCR analysis of the bound sialyllactose-DNA is then used to detect low attomolar concentrations of BoNT and attomolar to femtomolar concentrations of BoNT in honey, the most common foodborne source of infant botulism.
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