I have been trying to produce exosomes from platelets activated with thrombin. I usually get high yields after ultracentrifugation. However, the exosome pellets are very hard to resuspend and visually I can still see aggregates in the resuspension no matter how hard I try. Aggregation gets worse after storing in -80 freezers. I really need some advice here before moving on to other experiments.
Tarun Tyagi
Hi Tuan, You can try adding DMSO to your buffer before spin. I am not sure if that will adversely affect your downstream steps or not; but this can likely reduce aggregates i think.
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Hans-Jürgen Kolde
TRy TRAP instead of thrombin. TRAP does not activate the coagulation system.
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