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Run assay, Run assay 17, Considerations – Bio-Rad Human MMP and TIMP Assays User Manual

Page 19: Considerations when using a vacuum manifold

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8. Run Assay

Considerations

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Bring all buffers, diluents, diluted standards, diluted coupled beads, and

samples to room temperature before use

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

pipet tip for every volume transfer

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

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

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Assay incubations are carried out in the dark at 850 ± 50 rpm. Cover

the plate with sealing tape and protect from light with aluminum foil

Table 7. Summary of wash steps and incubations. 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

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

apparatus and remove the liquid by vacuum filtration

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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

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

between each vacuum step to prevent cross contamination

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

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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

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Bio-Plex Pro

Handheld Magnet or

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
Detection Ab incubation

MAG x3

VAC x3

3 x 100 μl

SA-PE incubation