User guide

3. Vortex the 20x stock of coupled beads at medium speed for

30 sec. Carefully open the cap and pipet any liquid trapped in the

cap back into the tube. This is important to ensure maximum bead

recovery. Do not centrifuge the vial; doing so will cause the

beads to pellet.

4. Dilute coupled beads to 1x by pipetting the required volume into the

15 ml tube. Vortex.

Each well of the assay requires 2.5 l of the 20x stock adjusted to a

ﬁnal volume of 50 l in assay buffer.

5. Protect the beads from light with aluminum foil. Equilibrate to room

temperature prior to use.

Note: To minimize volume loss, use a 200–300 l capacity pipet to remove

beads from the 20x stock tube. If necessary, perform the volume transfer in

two steps. Do not use a 1,000 l capacity pipet and/or wide bore pipet tip.

Preparing 1x coupled beads from 20x stock (includes 20% excess volume)

Table 6. Premixed panel or one singleplex assay.

Table 7. Mixing singleplex assays.

# of Wells 20x Beads, µl Assay Buffer, µl Total Volume, µl

96 288 5,472 5,760

48 144 2,736 2,880

20x Beads, µl 20x Beads, µl

# of Wells Singleplex #1 Singleplex #2 Assay Buffer, µl Total Volume, µl

288 288 5,184 5,760

144 144 2,592 2,880