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JoVE Encyclopedia of Experiments
Encyclopedia of Experiments: Immunology

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A Snap Chip Technology for a Cross-Reactivity-Free Multiplexed Sandwich Immunoassay

 

A Snap Chip Technology for a Cross-Reactivity-Free Multiplexed Sandwich Immunoassay

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To begin the immunoassay, remove the prepared assay slide from the freezer and allow it to warm to room temperature in its sealed bag for 30 minutes. Prepare seven serially diluted solutions of proteins in PBS with 0.05% polysorbate-20. Prepare appropriately diluted sample solutions in the same buffer.

Clamp a 24-well silicone gasket onto the room-temperature assay slide. Load the seven protein dilutions into seven of the eight wells in a column. Load protein-free PBS with 0.05% polysorbate-20 into the last well of that column. Load the sample solutions into the remaining wells.

Shake the slides at 450 RPM for 1 hour at room temperature or at 4 degrees Celsius overnight. Then, wash the slide three times. Remove the gasket and dry the slide under a stream of nitrogen gas.

Next, allow the detection antibody transfer slide to warm to room temperature for 30 minutes in its sealed bag. Then, incubate the slides for 20 minutes in a closed chamber with a relative humidity of 60% to rehydrate the arrays. Use the pogo pins to fix the detection transfer slide face-up in the snap apparatus.

Place the assay slide face-down on the pogo pins, and align the slide with the straight pins. Close the apparatus and snap-transfer the detection antibodies to the assay slide. Remove the slides from the apparatus and incubate the assay slide for one hour.

Clamp a 24-well silicone gasket to the slide, and wash the slide three times. Then, load into each well 80 microliters of a 2.5 microgram per milliliter solution of streptavidin fluorophore in PBS. Shake the slide at 450 RPM for 20 minutes.

Wash the slide three times with a 0.1% solution of polysorbate-20 in PBS, and once with distilled water. Then, remove the gasket and dry the slide. Scan the slide with a fluorescent scanner and measure the spot intensities. Determine the limits of detection and the protein concentrations.

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