Bio-Rad Mouse Typer Isotyping Kit User Manual

Note: When assessing color development using Model 3550,
Model 550, or the Model 3550-UV Microplate Reader, wash
the bottom of the assay plate thoroughly with distilled water
and wipe dry with non-lint toweling.

Section 3
Troubleshooting Guide

Problem

Probable Cause

Recommended Solution

A. High back-

1. Insufficient washing

1. Wash each well 6-7x and

ground.

after conjugate anti-

increase soak cycles to 30

body incubation.

seconds.

2. Insufficient blocking

2. Increase blocking step to

after antigen adsorption.

60 minutes.

3. Tween 20 absent from 3. Include Tween 20 in all

washes.

washes and solutions after
blocking.

4. GAR-HRP conjugate

4. Use recommended

concentration too high.

dilutions. Generally, the
less dilute, the higher the
background.

5. Color developed too

5. Decrease color develop-

long.

ment time by one-half.

6. Substrate too old (high 6. Use fresh solution A and

green color at working

solution B

dilution).

7. Whole cell antigens

7a. Use extracted antigens.

have endogenous

7b. Use other enzyme con-

peroxidase activity.

jugated antibodies.

7c. Destroy endogenous

activity by incubating
adsorbed Ag with mix-
ture of methanol/ H

2

O

2

(99 ml methanol, 1 ml
30% H

2

O

2

), 100 µl/well

for 1 hr.

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