|
1. Cell
Plating � no Test Reagent/Drug
(skip step 3 below) |
� Seed cells at 1-2 x 105
cells/ml, 100 ml/well |
2. Cell Plating �
withTest Reagent/Drug
(see below step 3) |
� Seed cells at 0.5-4 x
105 cells/ml, 50 ml/well |
|
3. Addition of Test
Reagent(s)/Drug |
� Add 50 ml/well, 2X
concentration desired |
|
4. Addition of BrdU
|
� Dilute 500X stock BrdU,
add 20 ml/well
(be sure to include a No BrdU control) |
|
5. Incubate |
� 2-24 hours |
6. Fix and Denature
- Adherent Cells
|
� Aspirate (or flick) the media from the cell wells
� Add 200 ml/well Fixing Solution
� Incubate 30 minutes at Room Temp.
� Aspirate the Fixing Solution and blot the plates dry.
|
- Suspension Cells
No-Spin Procedure |
� Add 200 ml/well Fixing
Solution on top of the cells.
� Incubate 1 hour at Room Temp
� Aspirate the Fixing Solution and blot the plates dry. |
- Suspension Cells
Spine Procedure |
� Spin the plates for 5
minutes at 1000 rpm.
� Aspirate media, add 200 ml/well Fixing Solution.
� Incubate for 30 minutes, room temp.
� Aspirate the Fixing Solution and blot the plates dry.
|
|
7. Wash Step |
� Wash X3 with 1X wash
buffer and blot dry. |
|
8. Detector Antibody
|
� Add 100 ml/well of
diluted detector antibody. |
|
9. Incubate |
� 1 hour at room temp. |
|
10. Wash Step
|
� Wash X3 with 1X wash
buffer and blot dry. |
|
11. Conjugate Addition
|
� Add 100 ml/well HRP-conjugate |
|
12. Incubate |
� Incubate for 30 minutes
at room temperature. |
|
13. Wash Step and Final
Water Wash |
� Wash as above. Perform
a final distilled water wash by flooding the entire
plate with distilled water. Pat dry on absorbent paper
towels. |
14. Development
|
� Add 100 ml/well
chemiluminescent substrate |
|
15. Read |
� Read immediately
(reaction may be read for up to 30 minutes). |
