Run assay, Run assay 22, Considerations – Bio-Rad Rat Diabetes Assays User Manual

22

7. Run Assay

Considerations

n

Bring all assay components and samples to room temperature before use

n

Use calibrated pipets and pipet carefully, avoiding bubbles. Use new

pipet tips for every volume transfer

n

Pay close attention to vortexing, shaking, and incubation instructions.

Deviation from the protocol may result in low assay signal and
assay variability

n

Assay incubations are carried out in the dark on a shaker at

850 ± 50 rpm. Cover the plate with sealing tape and protect from
light with aluminum foil

Table 13. Summary of wash options and protocols. After each assay step, select the
appropriate Bio-Plex Pro

™

wash station program or perform the appropriate manual wash step

as summarized below.

Considerations When Using a Vacuum Manifold

n

After each incubation, place the filter plate on a calibrated vacuum

apparatus and remove the liquid by vacuum filtration

n

To wash, add 100 μl wash buffer to each well and remove the liquid as

before. Ensure that all wells are exposed to the vacuum

n

Thoroughly blot the bottom of the filter plate with a clean paper towel

between each vacuum step to prevent cross contamination

n

Place the assay plate on the plastic plate holder/tray as needed

n

Before each incubation, gently cover the plate with a new sheet of

sealing tape. Avoid pressing down over the wells to prevent leaking
from the bottom

Bio-Plex Pro or

Bio-Plex Pro II

Handheld Magnet or

Pro II Wash Station

Wash Station

Vacuum Manifold

Assay Step

Magnetic Program

Vacuum Program

Manual Wash Steps

Add beads to plate

MAG x2

VAC x2

2 x 100 μl

Sample incubation

MAG x3

VAC x3

3 x 100 μl

Detection Ab incubation

MAG x3

VAC x3

3 x 100 μl

SA-PE incubation

MAG x3

VAC x3

3 x 100 μl