Thank your for your time.
0
2 replies to this topic
#1
zhaer
-
- Members
-
- 4 posts
member
0
Neutral
Neutral
Posted 28 January 2009 - 03:39 PM
I used a 5% separating with a 3% stacking and run for 90 min in total at 50 mA (constant). Gel was fixed in acetic acid/ethanol solution, stained by Coomassie Blue R-250. most of bands even markers (1st left lane)appear as two bands which seem from one protein. I'm very confused with what reason lead to band split.
Thank your for your time.
Thank your for your time.
#2
pesji
-
- Active Members
-
- 39 posts
Enthusiast
0
Neutral
Neutral
Posted 29 January 2009 - 05:52 AM
Maybe a problem with your buffer 
are you using SDS PAGE classical or MES buffers ?
are you using SDS PAGE classical or MES buffers ?
#3
zhaer
-
- Members
-
- 4 posts
member
0
Neutral
Neutral
Posted 29 January 2009 - 06:03 AM
pesji, on Jan 29 2009, 09:52 AM, said:
Maybe a problem with your buffer are you using SDS PAGE classical or MES buffers ?
are you using SDS PAGE classical or MES buffers ?I use classical SDS-PAGE buffer, do you mean it has a problem on buffer pH? I checked when I made them at room temperature, Stock stacking and separating solution are pH 6.8 and 8.8 respectively. Maybe I need to make a double check.
Edited by zhaer, 29 January 2009 - 06:06 AM.
