Multiplex Immunoassays

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Overview

For almost 50 years, immunoassays have allowed sensitive and highly specific detection of analytes of interest in biological samples for use in both life science research and clinical diagnostics. Traditional enzyme-linked immunosorbent assays (ELISA assays) detect and measure a single analyte per plate. Newer bead-based immunoassays, like those based on Luminex xMAP technology, utilize the same principle and apply it to uniquely identifiable beads. These beads allow for the simultaneous detection of multiple analytes in a single well or reaction. Multiplex immunoassays yield a wealth of information on the roles of multiple proteins and other biomolecules in diverse biological processes, thereby providing clinicians with insight into the identification and assessment of disease progression.

Early Immunoassays

The first immunoassay was developed by Yalow and Berson (1960), who received the Nobel Prize for their efforts to measure insulin levels. These initial assays used radiolabels for detection. The radioimmunoassay (RIA) would remain the standard for the detection of bioanalytes for more than ten years because of its extraordinary sensitivity, despite the health risks and disposal issues posed by the use of radioisotopes. The search for a suitable alternative to the RIA led to the development of ELISA in the early 1970s (Engvall and Perlmann 1971, Van Weeman and Schuurs 1971). ELISA uses an enzymatic reaction as the basis of detection, rather than a radioactive signal. While early versions did not rival the sensitivity of the RIA, the development of highly specific monoclonal antibodies and chemiluminescence detection resulted in ELISA assays with sensitivity that exceeds that of radiolabels. Today, key advantages of ELISA are its ease of use, flexibility, and low cost. The impact of immunoassays on life science research and clinical diagnostics has been enormous, with almost 10,000 studies published per year that include the terms “enzyme immunoassay” and “enzyme-linked immunoassay” (Lequin 2005). The growth of proteomics and genomic analysis is driving the need to discover and monitor large numbers of biomarkers indicative of human disease states. The output of the Human Genome Project, for example, provides the ability to simultaneously monitor the roles of multiple genes during investigations of complex biological systems.

Principles of Bead-Based Multiplex Immunoassays

The Bio-Plex® multiplex immunoassay system utilizes xMAP technology licensed from Luminex to permit the multiplexing of up to 100 different assays within a single sample. This technique involves 100 distinctly colored bead sets created by the use of two fluorescent dyes at distinct ratios. These beads can be further conjugated with a reagent specific to a particular bioassay. The reagents may include antigens, antibodies, oligonucleotides, enzyme substrates, or receptors. The technology enables multiplex immunoassays in which one antibody to a specific analyte is attached to a set of beads with the same color, and the second antibody to the analyte is attached to a fluorescent reporter dye label. The use of different colored beads enables the simultaneous multiplex detection of many other analytes in the same sample. A dual detection flow cytometer is used to sort out the different assays by bead colors in one channel and determine the analyte concentration by measuring the reporter dye fluorescence in another channel (Figure 1).

Illustration of antibody-conjugated fluorescent bead-based assay

Fig 1. Multiplex immunoassay technology. Beads are colored internally with two different fluorescent dyes (red and infrared). Different concentrations of red and infrared dyes are used to generate up to 100 distinct bead regions. Each bead region is conjugated to a specific target analyte (a) followed by binding with a biotinylated detection antibody (b) and a reporter dye, streptavidin-conjugated phycoerythrin (c).

During data acquisition, the contents of each microplate well are drawn into the array reader, depending on the type of reader — either the flow cytometry/laser excitation–based Bio-Plex 200 and Bio-Plex 3D systems or the light emitting diode (LED)/image-based analysis employed in the Bio-Plex® MAGPIX™ multiplex reader. For the flow cytometry–based systems, precision fluidics align the beads in single file through a flow cell where two lasers excite the beads individually. The red classification laser excites the dyes in each bead, identifying its spectral address. The green reporter laser excites the reporter molecule associated with the bead, which allows quantitation of the captured analyte. With the LED/image-based Bio-Plex MAGPIX reader, the beads are drawn into a chamber and magnetically immobilized. Classification and reporter excitation is accomplished with the use of LEDs rather than lasers. In all readers, high-speed digital signal processors and software record the fluorescent signals simultaneously for each bead, translating the signals into data for each bead-based assay (Figure 2).

Comparison of a traditional flow cytometry–based system with LED/image-based system

Fig 2. Data acquisition and reduction. Dyed beads are pushed through a detection chamber in a single file or magnetically immobilized. The red classification laser (635 nm) or LED interrogates the internal dyes to identify bead regions. The green reporter laser (532 nm) or LED interrogates the fluorescent reporter to measure analyte concentration.

 

Luminex xMAP Technology and Other Multiplex Immunoassays Techniques

Luminex xMAP technology is frequently compared to the traditional ELISA technique, which is limited by its ability to measure only a single analyte. The inability of traditional ELISA to multiplex presents additional limitations in sampling volume, cost, and labor (Figure 3). While the basic concepts of detection are similar between ELISA and Luminex xMAP technology, there are some important differences that center mainly on the capture antibody support. Unlike with traditional ELISA, Luminex xMAP capture antibodies are covalently attached to a bead surface, effectively allowing for a greater surface area as well as a matrix or free solution/liquid environment to react with the analytes. The suspended beads allow for assay flexibility in a singleplex or multiplex format.

Side-by-Side Comparison: Analyzing 27 Cytokines in 80 Samples

  ELISA Bio-Plex
Number of cytokines 27 27
Number of samples 80 80
Total data points 2,160 2,160
Number of 96-well plates 27
Stack of 27 96-well plate immunoassays
1
One 96-well plate immunoassay
Data points per plate 80 2,160
Total time required >60 hr 3 hr
Sample volume Serum or plasma, >1 ml*
Cell culture supernatant, >1 ml*
Serum or plasma, 12.5 μl
Cell culture supernatant, 50 μl
Assay range Serum or plasma, 2–3,000 pg/ml
Cell culture supernatant, 2–3,000 pg/ml
Serum or plasma, ~0.2–3,200 pg/ml
Cell culture supernatant, ~2–32,000 pg/ml

Fig 3. Protocol comparison between traditional ELISA and Bio-Plex system.

* Based on 50 µl/well sample

References

Engvall E and Perlmann P (1971). Enzyme-linked immunosorbent assay (ELISA). Quantitative assay of immunoglobulin G. Immunochemistry 8, 871–874.

Leguin RM (2005). Enzyme immunoassay (EIA)/enzyme-linked immunosorbent assay (ELISA). Clin Chem 51(12), 2415–2418.

Van Weeman, BK and Schuurs AH (1971). Immunoassay using antigen-enzyme conjugates. FEBS Lett 15(3), 232-236.

Yalow RS and Berson SA (1960). Immunoassay of endogenous plasma insulin in man. J Clin Invest 39, 1157-1175.

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Literature
Number Description Download
5297 Bio-Plex Cytokine Assay References, Rev C Click to download
5405 Bio-Plex Multiplex System Brochure, Rev D Click to download
5613 Bio-Plex Manager System Software Brochure, Rev B Click to download
6458 Bio-Plex Success Guide/Assay Sample Prep, Rev B Click to download
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