I am trying to purify protein having molecular weight ~50Kda under denaturing condition through Ni-NTA chromatography and got following profile. Any suggestion to stop protein coming in flow through and not binding with column.

conditions are 

protein dissolved in buffer-A (tris 50mM Urea 8M, Nacl-300mM)- for loading the sample on column.

column washed with same buffer supplemented with 60mM Imidazole.

and then eluted using imidazole linear gradient from 60-800mM Imidazole in Buffer-A

Bands are-

 GEL-1

Lane 1- marker

Lane 2-10 is elution during gradient

GEL-2

Lane 1- marker

Lane 2-8 is elution during gradient

Lane-9 flow through collected at the time of sample loading on column

Lane-10 -washing flow through of column by buffer A supplemented with 60mM Imidazole.  

Image -3 FPLC profile

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