Sample Processing for Assays

The Facility for Geroscience Analysis has standard preparation steps for its samples. Below are the preparation steps and information for urine, serum, and platelet-poor plasma. Also, each preparation type has a downloadable pdf version of the figure and steps. If you have any questions, please contact us.

Urine Preparation

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Step 1: After collection, keep urine refrigerated/on ice until processed.

Step 2: Transfer urine to a clean tube.

Step 3: Centrifuge the urine tube at 1400 x g for 10 minutes at 4°C

Step 4a: Transfer urine supernatant to a new clean tube

Step 4b: Cell pellet can be saved for future use. It contains cells and other elements.

Step 5: Aliquot urine supernatant into 1.5ml aliquots until the sample is exhausted.

Step 6: Store Aliquots at -80 °C until used.

Serum Preparation

Serum can be prepared from whole blood when collected on a tube without anticoagulant, containing or not clot activator. The blood clot can also be collected and frozen for future assays as it is a good source of DNA without preservatives.

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Step 1: After the blood draw, keep the blood tube at room temperature for 30 minutes to allow clot formation.

Step 2: Centrifuge the blood tube at 2000 x g for 10 minutes at 4°C

Step 3a: Transfer the serum supernatant to a new clean tube and mix by inverting five times

Step 3b: Optionally the blood clot can be transferred to a new tube and frozen for future use.

Step 4: Aliquot serum into 0.5ml aliquots until the sample is exhausted.

Step 5: Store Aliquots at -80 °C until used

Platelet Poor Plasma Preparation and Buffy Coat Preparation

Platelet-poor plasma and buffy coat can be prepared from whole blood with EDTA, Heparin, or Citrate/ACD as an additive. Buffy coat can be prepared for future use of live cells or not, depending on the assay to be run with those samples.

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Platelet-Poor Plasma Preparation

Step 1: After the blood draw, keep/transport blood tube refrigerated/on ice until processed.

Step 2: Centrifuge at 2000 x g for 10 minutes at 4°C

Step 3a: Transfer plasma to a new tube

Step 3b: Collect buffy coat

Step 4: Centrifuge plasma tube at 2000 x g for 10 minutes at 4°C

Step 5: Transfer Plasma Supernatant to new tube Mix by inverting 5 times.

Step 6: Aliquot EDTA/Hep platelet-poor plasma into 0.5ml aliquots until the sample is exhausted.

Buffy Coat Preparation

Step 3b: Transfer Buffy Coat into a 1.5 ml cryovial (Note: If no live cells are needed, freeze the tube at this time)

Step 3c: Add an equal volume of Freezing media and aliquot into two cryovials.

Step 3d: Slow-freeze overnight at -80 oC

Step 3e: Store in liquid Nitrogen