Bio-Rad Bio-Plex Pro™ RBM Canine Kidney Toxicity Assays User Manual

B. Dilution of Standard (1:3 Serial Dilution)

1. Label 8 polypropylene tubes S1 through S8.

2. Transfer the reconstituted standard into the tube labeled “S1.”

3. Add the appropriate amount of the standard diluent into the labeled

tubes according to the table below (this will be sufficient for duplicate
standard curves and blanks).

4. Prepare working standards (S2–S8) by serial dilution. Transfer the

appropriate volume of standard into each of the labeled tubes with
standard diluent as outlined above.

5. Vortex each standard at a medium setting before proceeding with the next

serial dilution. Change pipet tip at each dilution step.

C. Sample Preparation

1. Centrifuge samples at 500 x g for 5 min to remove particulates from all

samples prior to use.

2. Prepare sample dilutions in 0.5 ml or 1.0 ml polypropylene tubes as

required for the assay.

3. Dilution scenarios provided below are sufficient to run each sample

in duplicate.

Bio-Plex Pro Assay Quick Guide

Bio-Plex Pro Assay Quick Guide

Standard

Volume of Standard Diluent, µl

Volume of Standard, µl

S2

100

50 of S1

S3

100

50 of S2

S4

100

50 of S3

S5

100

50 of S4

S6

100

50 of S5

S7

100

50 of S6

S8

100

50 of S7

Blank

100

—

D. Dispensing of Reagents

1. Add 10 µl of blocker to all wells of the plate.

2. Add 30 µl of the standard, control, sample, or blank to the appropriate well

of the plate.

3. Vortex the capture beads at medium speed for 10–20 sec. Add 10 µl of the

beads to all wells of the plate.

4. Cover plate with plate seal and protect from light with aluminum foil.

Incubate on shaker at 850 ± 50 rpm for 1 hr at RT.

5. Wash the plate three times with 100 µl 1x assay buffer.

6. Vortex the reconstituted detection antibodies at medium speed for

10–20 sec. Add 40 µl to each well.

7. Cover and incubate at 850 ± 50 rpm, as in Step 4, for 1 hr at RT. Do not

aspirate after incubation.

8. Prepare the required dilution of SA-PE as outlined in the following table.
Note: Volumes in the table are for an entire 96-well plate. Smaller volumes

can be prepared, provided that dilution ratios are maintained.

9. Add 20 µl of diluted SA-PE to the required plate wells.

Volume of

Volume of

Panel

Sample Dilution

Urine Sample, µl

Sample Buffer, µl

Human Tox 1

1:4

20

60

Human Tox 2

1:50

10

490

Rat Tox 1

1:2

40

40

Rat Tox 2

1:50

10

490

Rat Albumin

1:10,000

5 (A. Prepare 1:100)

495

5 (B. Prepare 1:100)

495

Canine Tox 1

1:15

10

140

Canine Albumin 1:10,000

5 (C. Prepare 1:100)

495

5 (D. Prepare 1:100)

495

Note: Controls are ready to use after reconstitution. No dilution is needed.