Citation

BibTex format

@article{McDonald:2016:10.1016/j.jim.2016.02.018,
author = {McDonald, JU and Ekeruche-Makinde, J and Ho, MM and Tregoning, JS and Ashiru, O},
doi = {10.1016/j.jim.2016.02.018},
journal = {Journal of Immunological Methods},
pages = {6--16},
title = {Development of a custom pentaplex sandwich immunoassay using Protein-G coupled beads for the Luminex® xMAP® platform.},
url = {http://dx.doi.org/10.1016/j.jim.2016.02.018},
volume = {433},
year = {2016}
}

RIS format (EndNote, RefMan)

TY  - JOUR
AB - Multiplex bead-based assays have many advantages over ELISA, particularly for the analyses of large quantities of samples and/or precious samples of limited volume. Although many commercial arrays covering multitudes of biologically significant analytes are available, occasionally the development of custom arrays is necessary. Here, the development of a custom pentaplex sandwich immunoassay using Protein G-coupled beads, for analysis using the Luminex® xMAP® platform, is described. This array was required for the measurement of candidate biomarkers of vaccine safety in small volumes of mouse sera. Optimisation of this assay required a stepwise approach: testing cross-reactivity of the antibody pairs, the development of an in-house serum diluent buffer as well as heat-inactivation of serum samples to prevent interference from matrix effects. We then demonstrate the use of this array to analyse inflammatory mediators in mouse serum after immunisation. The work described here exemplifies how Protein G-coupled beads offer a flexible and robust approach to develop custom multiplex immunoassays, which can be applied to a range of analytes from multiple species.
AU - McDonald,JU
AU - Ekeruche-Makinde,J
AU - Ho,MM
AU - Tregoning,JS
AU - Ashiru,O
DO - 10.1016/j.jim.2016.02.018
EP - 16
PY - 2016///
SN - 1872-7905
SP - 6
TI - Development of a custom pentaplex sandwich immunoassay using Protein-G coupled beads for the Luminex® xMAP® platform.
T2 - Journal of Immunological Methods
UR - http://dx.doi.org/10.1016/j.jim.2016.02.018
UR - http://hdl.handle.net/10044/1/31726
VL - 433
ER -