4.8 Article

Four Assay Designs and On-Chip Calibration: Gadgets for a Sepsis Protein Array

Journal

ANALYTICAL CHEMISTRY
Volume 86, Issue 6, Pages 3174-3180

Publisher

AMER CHEMICAL SOC
DOI: 10.1021/ac5000784

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Funding

  1. Austrian Research Promotion Agency (FFG) of the MNT Era Net Project Valipro within the Austrian NANO Initiative Programme Action Line Transnational Cooperative RTD Projects [823977]

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A protein microarray for the early stage diagnosis of sepsis that allows the simultaneous detection of C-reactive protein (CRP) (2-200 mu g/mL), procalcitonin (PCT) (0.2-50 ng/mL), and interleukin 6 (IL-6) (2-2000 pg/mL) has been developed. To enable the parallel detection of the differently abundant analytes, the low binding affinity between CRP and phosphocholine is exploited in a low-sensitive sandwich assay for CRP. The calibration is integrated directly on the chip resulting in a one patient one array format, to provide a user-friendly and rapid diagnostic tool. Four different assay designs are introduced: (I) the classical assay that works with biotin streptavidin chemistry, (II) the rapid assay that is performed in a single detection step, and two ultrasensitive assay designs accomplished either by (111) an enzymatic or (IV) an antibody mediated amplification resulting in high density labeling. The assay designs were evaluated by the repetitive measurement of low, medium, and high concentration levels of commercially available certified control sera. The precision was similar across all assay designs (coefficient of variation (CV), CVintra 8-14%; CVinter : 18-34%), while the sensitivity (limits of detection (LODs)) increased by I order of magnitude for the ultrasensitive assays (III, IV) and the accuracy was analyte dependent but best for the classical (I) and the antibody amplified (IV) assays.

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