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I am newbie in PAGE and this is my first experience conducting Native-PAGE, particularly.Actually, this is as a preliminary experiment before conducting the IEF. I try to load the genomic DNA in 7.5% Acrylamide gel with the below recipes:
Bis-acry (30%)
4x resolving 15 ml
APS 25% = 120 uL
TEMED = 10 uL
The Anode Buffer = 0.45M Tris/Acetate; 4 g/L SDS. pH: 6.6
The Cathode Buffer = 0.08 M Tris; 6 g/L SDS. pH: 7.1 (actually, the recommendation is added with 0.80 Tricine. But, I omit it coz, my lab doesn’t have the available one )
I utilized the Flatbed-Multiphor III Electrophoresis System (GE ). I run the gel for 5h, 200V and 15ºC. The genome DNA that Ive loaded were 1 ng/uL, so I visualized with silver staining method. But, after several time Ive conducted this experiment. I can not see my band and I found my band was faint smear. Early, I thought it was caused by the voltage. So, I decrease the voltage to 200V. but, seems it disaster appear again in the same way.
Ive included the image. The left side of lane was the Lambda DNA marker but the phenomenon was similar with the other well. Please…, Please give me some suggestions to solve this problem!! I am desperate!!
