I 'm performing a lot of indirect ELISA assays to assess IgG in human blood on DBS. In general, I have to use 0.1% Tween 20 in PBS buffer to elute my DBS. This is going great. But I recently received DBS made with the same paper (Whatman 3M), on which drop of blood does not elute although I used the same protocol (even incubated for more than 48 hours).
However, it's important to tell that this DBS were stored for a long time at room temperature, but just under the air conditioner (instead of at 4°C as usually).
Please, could anyone with experience on elution of DBS give me any ideas?
I apologize for the omission, DBS correspond to Dried Blood Spot.
Assuming that the stability/variance in recovery was tested this should not be a problem of elution. Most likely it is a problem of stability, as you mentioned storage under the air conditioner. This can easily be tested by placing a known sample in the same place and consecutive analysis.
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