Aqueous two-phase system patterning of detection antibody solutions for cross-reaction-free multiplex ELISA

Frampton, John P.; White, Joshua B.; Simon, Arlyne; Tsuei, Michael; Paczesny, Sophie; Takayama, Shuichi

doi:10.1038/srep04878

Cited by 54 publications

(58 citation statements)

References 43 publications

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“…More recently, ATPS has been used to generate multiplex antibody-based assays [58,59]. Importantly, many antibodies demonstrate strong partitioning to the dextran phase in an ATPS composed of polyethylene glycol and dextran (K≪1).…”

Section: Spatially-patterned Multiplexing For Multiple Tissue Regionsmentioning

confidence: 99%

Recent developments in multiplexing techniques for immunohistochemistry

Dixon

Bathany

Tsuei

et al. 2015

Expert Review of Molecular Diagnostics

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102

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Methods to detect immuno-labelled molecules at increasingly higher resolution, even when present at low levels, are revolutionizing immunohistochemistry (IHC). These technologies can be valuable for management and examination of rare patient tissue specimens, and for improved accuracy of early disease detection. The purpose of this mini-review is to highlight recent multiplexing methods that are candidates for more prevalent use in clinical research and potential translation to the clinic. Multiplex IHC methods, which permit identification of at least 3 and up to 30 discrete antigens, have been divided into whole section staining and spatially-patterned staining categories. Associated signal enhancement technologies that can enhance performance and throughput of multiplex IHC assays are also discussed. Each multiplex IHC technique, detailed herein, is associated with several advantages as well as tradeoffs that must be taken into consideration for proper evaluation and use of the methods.

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Section: Spatially-patterned Multiplexing For Multiple Tissue Regionsmentioning

confidence: 99%

Recent developments in multiplexing techniques for immunohistochemistry

Dixon

Bathany

Tsuei

et al. 2015

Expert Review of Molecular Diagnostics

Self Cite

102

View full text Add to dashboard Cite

show abstract

“…To mitigate risks of cross-reactions, tedious systematic evaluations of nonspecific interactions between each antibody and each measured protein must be performed to validate these assays 7–10 . Alternatively, matched capture and detection antibody pairs can also be co-localized 11,12 . Multiplexing AlphaLISA™ is even more challenging because single-color signals, generated by homogeneously distributed antibody-bead reagents, cannot be spatially localized within one well or spectrally resolved using conventional methods.…”

Section: Introductionmentioning

confidence: 99%

Aqueous two-phase systems enable multiplexing of homogeneous immunoassays

et al. 2014

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Quantitative measurement of protein biomarkers is critical for biomarker validation and early disease detection. Current multiplex immunoassays are time consuming costly and can suffer from low accuracy. For example, multiplex ELISAs require multiple, tedious, washing and blocking steps. Moreover, they suffer from nonspecific antibody cross-reactions, leading to high background and false-positive signals. Here, we show that co-localizing antibody-bead pairs in an aqueous two-phase system (ATPS) enables multiplexing of sensitive, no-wash, homogeneous assays, while preventing nonspecific antibody cross-reactions. Our cross-reaction-free, multiplex assay can simultaneously detect picomolar concentrations of four protein biomarkers ((C-X-C motif) ligand 10 (CXCL10), CXCL9, interleukin (IL)-8 and IL-6) in cell supernatants using a single assay well. The potential clinical utility of the assay is demonstrated by detecting diagnostic biomarkers (CXCL10 and CXCL9) in plasma from 88 patients at the onset of the clinical symptoms of chronic graft-versus-host disease (GVHD).

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“…In terms of general assay performance, this new multiplex assay platform is similar to standard single biomarker ELISA. Comparison data for limit of detection and linear dynamic range are reported in two recent publications that describe the antibody confinement technology [3,5].…”

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confidence: 99%

“…In a recent report that measured plasma biomarkers by ELISA for assessment of therapy-resistant GVHD [6], an average receiver operating characteristic area under the curve (AUC; which is a measure of the sensitivity and specificity of the test for various biomarker cutoff concentrations) of 0.78 was obtained for a set of 12 individual GVHD biomarkers. The polymer-based ELISA system yielded a slightly higher average receiver operating characteristic AUC of 0.85 for a set of four individual GVHD biomarkers using a smaller set of clinical samples [5].…”

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confidence: 99%

“…To address this limitation of multiplex immunoassays, an array-based immunoassay has recently been developed that eliminates the possibility of cross-reactions among antibodies in a multi-biomarker panel by confining the antibodies at specific sites on an assay plate [3][4][5]. Antibody confinement is enabled using polymer solutions that phase-separate from each other, much like oil droplets in water.…”

mentioning

confidence: 99%

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