I am trying to find a working protocol to label some proteins (commercially purchased) with carboxylate modified fluospheres (20 or 40 nm size). I figured out that this can be done using a EDC sulfo-NHS assisted conjugation. Though I could find some references, I have few concerns.

(1) My protein concentration (0.4 mg/ml) is low when compared to the references.

(2) Protein is stored in phosphate buffer but contains glycerol (50%), DTT (10 mM) and Triton-X (0.15 %) and I am not sure whether these have any influence on the reaction.

(3) The size of my fluospheres can't be larger than 40 nm.

(4) What kind of purification method will be suitable after the conjugation process?

Any suggestions?

Similar questions and discussions