Size exclusion filter purification

Folded samples BM_2_1565 (23.8.2011) and BM_2_5Dh3ml (23.8.2011) filtered in Amicon (100 kDa) with 0.5 TBE + 11mM MgCl2

Sample filtering

• 50 µl from both samples were mixed and put into a Amicon filter (100 kDa)
• 400 µl 0.5x TBE + 11mM MgCl2 added
• spinned for 5 minutes at 14000 rcf
• 400 µl 0.5x TBE + 11mM MgCl2 added
• spinned for 5 minutes at 14000 rcf
• 400 µl 0.5x TBE + 11mM MgCl2 added
• spinned for 5 minutes at 14000 rcf
• turned the filter and sinned the purified sample into a new Epi for 2 minutes at 1000 rcf
• 1 x and 2 x filtered buffer filled into separate Epi (the buffer, which came through the filter; if purification with spin columns works, this should only contain staples)
• 3 x timed filtered buffer discarded

Ran a 50 ml 2% Agarose-Gel with EtBr

wed

• 1kb ladder
• p7560
• filtered BM_2
• BM_2_1565
• BM_2_5Dh3ml
• 1x filtered buffer
• 2x filtered buffer

Gel picture

insert jpeg!!!

• looks like there are residual staples in solution and the leading band is slower as the scaffold. Marty said this is normal, when purified samples are put on a gel.
• new purification with less initial concentration and folding buffer as washing buffer
• look at samples in the TEM as soon as possible!!!

Folded sample BM_1_1565 (23.8.2011) in Amicon (100 kDa) with 1 x FOBXM + 20 mM MgCl2

Sample filtering

• 50 µl sample in a Amicon filter (100 kDa)
• 500 µl 1xFOBXM20 added
• spinned for 5 minutes at 14000 rcf
• 500 µl 1xFOBXM20 added
• spinned for 5 minutes at 14000 rcf
• 500 µl 1xFOBXM20 added
• spinned for 5 minutes at 14000 rcf
• turned the filter and sinned the purified sample into a new Epi for 2 minutes at 1000 rcf
• 1 x and 2 x filtered buffer filled into separate Epi (the buffer, which came through the filter; if purification with spin columns works, this should only contain staples)
• 3 x timed filtered buffer discarded

Ran a 125 ml 2% Agarose-Gel with EtBr