A Typical problem in column chemistry
Posted: Mon Jul 16, 2012 8:55 am
Hi,
I have a typical problem. I am analyzing proteins from fermentation supernatant and injecting around 5µl. I have connected a new column(ACE 300A 4.6X250mm;5µm) and injected my sample, i got gautian shape with lot of tailing.Then, i injected 200-300µl of the same sample supernatant in to the column and continued my regular injection volume.
After the Higher injection load to the column the usual injection samples is giving very good symmetrical peaks. can any one say what is really happening? Am i blocking any active sites by loading higher injection volume?.
Am i avoiding any secondary intreaction between solute and stationay phase?
If any one joins this discussion, it will be good to find out a answer for a new problem.
Thanks
vijayak
I have a typical problem. I am analyzing proteins from fermentation supernatant and injecting around 5µl. I have connected a new column(ACE 300A 4.6X250mm;5µm) and injected my sample, i got gautian shape with lot of tailing.Then, i injected 200-300µl of the same sample supernatant in to the column and continued my regular injection volume.
After the Higher injection load to the column the usual injection samples is giving very good symmetrical peaks. can any one say what is really happening? Am i blocking any active sites by loading higher injection volume?.
Am i avoiding any secondary intreaction between solute and stationay phase?
If any one joins this discussion, it will be good to find out a answer for a new problem.
Thanks
vijayak