ASTM WK69051
New Test Method for Assessing the Activation of the Complement System in Human Plasma Through Quantification of iC3b Concentration by ELISA,
1. Scope
The purpose of this assay is to determine complement activation by nanoparticles . Nanoparticles which may absorb within the assay range of the Enzyme Linked Immunosorbent Assay (ELISA) should be treated with caution due to interference. Inhibition/enhancement controls should always be included.Keywords
Nanoparticles, Enzyme, Immunosorbent, ELISA, complement, iC3b, plasmaRationale
The complement (C) system is a major contributor to innate immunity and is composed of more than 30 proteins. Three cascades (classical, lectin and alternative) may be activated by differing triggers resulting in the generation of complement component 3 (C3). In turn, particularly in the alternative pathway, C3 may further generate C3a and C3b. C3a acts as an anaphylotoxin that promotes inflammatory processes where C3b can be further cleaved to generate inactive C3b (iC3b) which has opsonic properties. Nanoparticles, and nanoparticulate surfaces, are known to activate the C system. Determination of C activation, ex vivo, by nanoparticles may provide information as to their biocompatibility and possible CARPAgenicity. This test method describe a protocol for the determination of C activation, in human plasma, by Enzyme Linked Immunosorbent Assay (ELISA) measurement of iC3b concentrations.
Work Item Status
Date Initiated: 07-11-2019
Technical Contact: Bryant Nelson
Item: 000
Ballot:
Status: