Hi all

I'm trying to perform the procedure of sickling-induction in-vitro of peripheral red blood cells from sickle cell Townes mice, and I'm using 2% sodium metabisulfite. Unfortunately the protocol doesn't seem to work perfectly, as sometimes I see quite a lot of sickling, yet other times I can't really see much or any at all. I always compare a sickle cell mouse with a normal human Hb mouse. I obtain blood from saphenous bleed; using a heparinized capillary tube I transfer the blood to a microtube containing 3-5 uL of heparin. The 2% sodium metabisulfite is freshly made within 30-60 minutes, resuspended in PBS. I mix 10 uL of sodium metabisulfite solution with 10 uL of heparinized blood, and then transfer 10 uL of the mix into a slide, which I cover and then seal with transparent nail polish. I incubate my slides for 45-60 minutes at 37C 5% CO2. I look at the slides under phase contrast microscopy.

Does anyone have a good idea how to make more consistent my sickling effect?

Thanks in advance!

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