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What is the typical assay set-up?

assay set-up
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What is the typical assay set-up?

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The plates or the tubes are delivered with the different concentration of TRANSIL beads. After compound addition, mixing and incubation for 2 minutes, beads are separated by low speed centrifugation (5 minutes with 750 g). A fixed volume of the final supernatant is transferred into a new plate for quantification either by UV, HPLC or LC/MS.

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