Nucleic acids extraction from single cell using MasterPure Complete DNA purification (Epicenter)

Isolate individually protist cells (at least 50µm in length) using a glass bent micropipette under a binocular microscope.

Wash each cell in three successive baths of 0.22µm-filtered and sterile seawater.

Transfer subsequently cells in a 1.5mL sterile microtube.

Add 30 μL of lysis buffer (Tissue and Cell Lysis Solution from MasterPureTM DNA and RNA Purification Kit, Epicenter) and store at -20°C.

Pellet cells by centrifugation (2 min at Vmax), throw the supernatant, let ~25-30 µL of liquid.

Dilute 1 µL of Proteinase K in 300 µL de lysis solution Tissue et Cellule for each sample. Vortex 10 sec for resuspending cells (facultative).

Add 300 µL of mix Proteinase K + lysis solution Tissue et Cellule in each sample. Vortex.

Incubate 15 min at 65°C , 1000 rpm. Put samples in ice 3-5 min.

Add 150 µL MPC reagent to 300 µL of lysed sample. Vortex.

Spin 10 min at 11 000 g, 4°C. If there is no pellet, add more 25 µL MPC buffer and spin again 10 min at 11 000 g, 4°C.

Transfer the supernatant ion a new clean microtube (1,5 mL), discard the pellet.

(To keep the squeletton, keep the tube with the pellet, add 500 µL MilliQ Water and store at -20°C).

Add 500 µL of Isopropanol. Mix per inversion. Spin 10min at Vmax, 4°C.

Discard the supernatant with precaution, without touching the pellet.

Add 500 µL of Ethanol 70%. Don’t vortex , mix gently the support. Spin 5min at Vmax ;at 4°C.

Discard a maximum of supernatant with precaution, without touching the pellet.

Let dry 5-10 min at room temperature. The pellet should become transparent.

Elute in 25 µL of TE1x buffer.

Vortex and spin shortly.

Store at - 80°C.