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Modification of sample processing for theLimulusamebocyte lysate assay enhances detection of inflammogenic endotoxin in intact bacteria and organic dust
Author(s) -
Kimberly A Hoppe Parr,
Suzana Hađina,
Brita KilburgBasnyat,
Yifang Wang,
Dulce Chavez,
Peter S. Thorne,
Jerrold Weiss
Publication year - 2017
Publication title -
innate immunity
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 0.921
H-Index - 69
eISSN - 1753-4267
pISSN - 1753-4259
DOI - 10.1177/1753425917694084
Subject(s) - limulus amebocyte lysate , bacteria , microbiology and biotechnology , chemistry , limulus , lipopolysaccharide , lysis , potency , escherichia coli , chromatography , tris , neisseria meningitidis , biochemistry , biology , in vitro , immunology , genetics , paleontology , gene
The pro-inflammatory potency and causal relationship with asthma of inhaled endotoxins have underscored the importance of accurately assessing the endotoxin content of organic dusts. The Limulus amebocyte lysate (LAL) assay has emerged as the preferred assay, but its ability to measure endotoxin in intact bacteria and organic dusts with similar sensitivity as purified endotoxin is unknown. We used metabolically radiolabeled Neisseria meningitidis and both rough and smooth Escherichia coli to compare dose-dependent activation in the LAL with purified endotoxin from these bacteria and shed outer membrane (OM) blebs. Labeled [ 14 C]-3-OH-fatty acids were used to quantify the endotoxin content of the samples. Purified meningococcal and E. coli endotoxins and OM blebs displayed similar specific activity in the LAL assay to the purified LPS standard. In contrast, intact bacteria exhibited fivefold lower specific activity in the LAL assay but showed similar MD-2-dependent potency as purified endotoxin in inducing acute airway inflammation in mice. Pre-treatment of intact bacteria and organic dusts with 0.1 M Tris-HCl/10 mM EDTA increased by fivefold the release of endotoxin. These findings demonstrate that house dust and other organic dusts should be extracted with Tris/EDTA to more accurately assess the endotoxin content and pro-inflammatory potential of these environmental samples.

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