Acute induction of anomalous and amyloidogenic blood clotting by molecular amplification of highly substoichiometric levels of bacterial lipopolysaccharide

Pretorius, Etheresia; Mbotwe, Sthembile; Bester, Janette; Robinson, Christopher J.; Kell, Douglas B.

dc.contributor.author	Pretorius, Etheresia
dc.contributor.author	Mbotwe, Sthembile
dc.contributor.author	Bester, Janette
dc.contributor.author	Robinson, Christopher J.
dc.contributor.author	Kell, Douglas B.
dc.date.accessioned	2017-02-01T06:44:18Z
dc.date.available	2017-02-01T06:44:18Z
dc.date.issued	2016
dc.description.abstract	It is well known that a variety of inflammatory diseases are accompanied by hypercoagulability, and a number of more-or-less longer-term signalling pathways have been shown to be involved. In recent work, we have suggested a direct and primary role for bacterial lipopolysaccharide (LPS) in this hypercoagulability, but it seems never to have been tested directly. Here, we show that the addition of tiny concentrations (0.2 ng l21) of bacterial LPS to both whole blood and platelet-poor plasma of normal, healthy donors leads to marked changes in the nature of the fibrin fibres so formed, as observed by ultrastructural and fluorescence microscopy (the latter implying that the fibrin is actually in an amyloid b-sheet-rich form that on stoichiometric grounds must occur autocatalytically). They resemble those seen in a number of inflammatory (and also amyloid) diseases, consistent with an involvement of LPS in their aetiology. These changes are mirrored by changes in their viscoelastic properties as measured by thromboelastography. As the terminal stages of coagulation involve the polymerization of fibrinogen into fibrin fibres, we tested whether LPS would bind to fibrinogen directly. We demonstrated this using isothermal calorimetry. Finally, we show that these changes in fibre structure are mirrored when the experiment is done simply with purified fibrinogen and thrombin (+0.2 ng l21 LPS). This ratio of concentrations of LPS : fibrinogen in vivo represents a molecular amplification by the LPS of more than 108-fold, a number that is probably unparalleled in biology. The observation of a direct effect of such highly substoichiometric amounts of LPS on both fibrinogen and coagulation can account for the role of very small numbers of dormant bacteria in disease progression in a great many inflammatory conditions, and opens up this process to further mechanistic analysis and possible treatment.	en_ZA
dc.description.department	Physiology	en_ZA
dc.description.librarian	am2017	en_ZA
dc.description.sponsorship	The Biotechnology and Biological Sciences Research Council (grant no. BB/L025752/1), the National Research Foundation (NRF) of South Africa and a contribution from the Manchester Centre for Synthetic Biology of Fine and Speciality Chemicals (SYNBIOCHEM) (BBSRC grant BB/M017702/1).	en_ZA
dc.identifier.citation	Pretorius E, Mbotwe S, Bester J, Robinson CJ, Kell DB. 2016 Acute induction of anomalous and amyloidogenic blood clotting by molecular amplification of highly substoichiometric levels of bacterial lipopolysaccharide. Journal of the Royal Society Interface 13: 20160539. http://dx.DOI.org/ 10.1098/rsif.2016.0539.	en_ZA
dc.identifier.issn	1742-5689 (print)
dc.identifier.issn	1742-5662 (online)
dc.identifier.other	10.1098/rsif.2016.0539
dc.identifier.uri	http://hdl.handle.net/2263/58756
dc.language.iso	en	en_ZA
dc.publisher	The Royal Society	en_ZA
dc.rights	© 2016 The Authors. Published by the Royal Society under the terms of the Creative Commons Attribution License.	en_ZA
dc.subject	Bacterial lipopolysaccharide	en_ZA
dc.subject	Plasma	en_ZA
dc.subject	Thromboelastography	en_ZA
dc.subject	Electron microscopy	en_ZA
dc.subject	Amyloid	en_ZA
dc.subject	Fibrin	en_ZA
dc.subject	Lipopolysaccharide (LPS)	en_ZA
dc.title	Acute induction of anomalous and amyloidogenic blood clotting by molecular amplification of highly substoichiometric levels of bacterial lipopolysaccharide	en_ZA
dc.type	Article	en_ZA