Photo-Oxidation of MiniSOG Related to Cultured Neurons

Plate cells in MaTek dishes.

Fix in 2.5% glutaraldehyde in 0.1 M cacodylate buffer at room temperature for 5 min. Then, for one hour on ice.

 **IMPORTANT: Keep Everything cold!** 

Wash 5x for 1 min in 0.1M cacodylate buffer.

Block for 30 min on ice with blocking buffer.

Wash 3x in 0.1M cacodylate buffer for 1 min.

Block in 5 – 10 mM mersalyl acid for 30 min.

Wash 3x for 1 min with 0.1M cacodylate buffer.

Remove solution from plate and replace with DAB solution.

At the microscope, set the temperature of the stage at 4˚C. Set the MaTek dish on the proper holder. Install oxygen, find target area with 63X objective lens, take initial picture (fluorescence + DIC).

Turn oxygen ON to blow onto surface of sample solution. (Regarding oxygenation: periodically replacing with freshly oxygenated solution is fine too when working with cultured cells).

Illuminate target area to photo-oxidize until light browning. Important: miniSOG is fast (2 to 10 minutes depending on protein). Optimal timing needs to be determined by investigator and will require the EM analysis of the samples at different reaction time.

Take final picture after photo-oxidation. Go to next area in the same dish and repeat, usually 3-4 areas per plate, making sure they are equally spaced to facilitate separation and cutting of individual blocks after polymerization.

When done, remove dish from holder, wash immediately 5x for 1 min in 0.1 M cacodylate buffer, on ice.

Fix in 1% osmium tetroxide in 0.1M cacodylate buffer. Leave 30 min on ice.

Wash 5x for 1 min in ddH₂O.

Optional step: Add filtered 2% UA (uranyl acetate) in ddH2O at 4˚C for 1hr on ice. Wash 5x for 1 min in ddH₂O.

Dehydrate: 20-50-70-90-100-100% cold Ethanol (1 min each). Then 100% dry ethanol at room temperature 3x for 1 minute.

Infiltration and Embedding: Prepare Durcupan: A:B:C:D=11.4:10:0.3:0.1 g

Add 50% ethanol: 50% Durcupan to dish. Leave for 30 min.

Pour out and add 100% Durcupan. Leave for 1 hour.

Add new 100% Durcupan resin, leave for 1 hr. Scrape out with a pair of plain wood applicators (Product No. 23-400-102 Fisherbrand) and without touching the cover slip containing the cells.

Add new 100% Durcupan resin, leave for 1 hr. Scrape out with a pair of plain wood applicators (Product No. 23-400-102 Fisherbrand) and without touching the cover slip containing the cells.

Add new 100% Durcupan resin, leave for 1 hr. Scrape out with a pair of plain wood applicators (Product No. 23-400-102 Fisherbrand) and without touching the cover slip containing the cells.

Add new 100% Durcupan resin, place in vacuum oven to polymerize for 48 hrs (60˚C).