Bio-Rad Rat Diabetes Assays User Manual

23

Add Coupled Beads, Standards, Blanks, Samples,

and Controls

1. Cover unused wells with sealing tape.

2. Prewet the filter plate. Skip this step if using a flat bottom plate.

a)

Prewet the wells with 100 µl of assay buffer and remove the liquid

by vacuum filtration. Dry the bottom of the filter plate thoroughly
by blotting on a clean paper towel.

3. Vortex the diluted (1x) coupled beads for 30 sec at medium speed.

Pour the diluted coupled beads into a reagent reservoir and transfer
50 µl to each well of the assay plate.

Tip: A multichannel pipet is highly recommended for ease of use

and

efficiency.

4. Wash the plate two times with 100 µl Bio-Plex wash buffer using

the wash method of choice.

5. Gently vortex the diluted standards, blanks, samples, and controls

(if applicable) for 5 sec. Transfer 50 µl to each well of the assay plate,
changing the pipet tip after every volume transfer

6. Cover plate with a new sheet of sealing tape and protect from light

with aluminum foil. Incubate on shaker at 850 ± 50 rpm for 1 hr at
room temperature (RT).

Note: 850 rpm provides equivalent performance to previously
recommended shaker settings (1,100 rpm for 30 sec, 300 rpm for
incubation).

Note: Be consistent with this incubation time for optimal assay
performance and reproducibility.