We found a small protein that we can aggregate, after purification. We do not believe them to be in their native state. So what properties of the elution/storage buffer can prevent/break protein (pure) aggregation. Does this have anything to do with the inherent properties of proteins? If yes, what are they? Can we understand the protein as such as we are not able to functionally characterize the protein at present, although we know the sequence characteristics. Where are we missing the catch, the monomer?