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I am desperate for help.
During SDS page:
I keep getting smear of my sample during loading. I loaded little sample of my protein of interest ( ~80kd) approx. 1000pg. in 10% seperating gel. I seems to have trouble getting a clear band. Could adding too much sample buffer be effecting the migration? As I used sample buffer to dilute my sample. ( When i used water the sample couldnt seems to sink into the well.
During Western blot:
I didnt even get a band or background signal on the X ray film?
my protocol was as below:
1. After transfering the proteins from the gel to nitrocellulose membrane at 40V overnight.
2. Stain the membrane with ponceu S.
3. Wash 2x with dH20
4. Wash 2x with TBS buffer
5. block with 5% milk for 1 hour at RT
6. Wash 2x with TBS buffer
7. Wash 1x with TBS T buffer
8. Primary AB (1/2000) for 2 hours
9. Wash 2x with TBS buffer
10. Wash 1x with TBS T buffer
11. Secondary Ab(1/2000) for 1 hour
12. React with chemiluminenece for 5 min ( blot membrane dry on both side)
13. Expose with X -RAy film..
No exposure.
Hopeful for a response?
so I believe theres something wrong with my technique..
