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H201 temperature unit

Manufactured by Okolab

The H201-Temperature Unit is a laboratory equipment product designed to regulate and maintain the temperature of samples or specimens in a controlled environment. It provides precise temperature control functionality without interpreting or extrapolating its intended use.

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2 protocols using h201 temperature unit

1

Calcium Imaging of Oligodendrocyte Processes

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Immunopanned CalEx; Cnp-Cre OPCs were differentiated for two to three days for all calcium imaging experiments. To load 1 μM cell permeable calcium indicator, Fluo-4-AM (Invitrogen, F14201) 50 μg tube of lyophilized Fluo-4-AM stock was resuspended in 46 uL of sterile DMSO (1 mM concentration). 1.5 μL of Fluo-4-AM stock was added directly to cell media to prevent shearing of cells. Cells were incubated with Fluo-4-AM for 20 minutes and then media was completely changed to 1 mL DMEM-SATO Media (made with Fisher Scientific A1896701) for imaging.
Cells were imaged on an Opterra II Multipoint Swept Field Confocal outfitted with a humidified, temperature-controlled microscope enclosure (Okolab microscope enclosure, H201-Temperature Unit, CO2 controller, HM-Active Vibration Free Humidity Controller with humidity sensor and temperature-controlled tube). Imaging was performed using the 60x/1.2 NA water objective and Perfect Focus to prevent z-plane drift during imaging. Images were acquired every two seconds in 488 channel with 70 μM slit and 100 ms exposure time with 15% laser power. Calcium imaging data was analyzed using Fiji to select regions of interest and was analyzed to extract rate and amplitude measurements. All calcium imaging was performed on oligodendrocyte processes; soma events were relatively rare compared to process events. Data was analyzed blind to condition.
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2

Live-cell imaging of neuronal responses

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Live-and fixed-cell widefield imaging was performed on an inverted Nikon Eclipse Ti2-E microscope For the live-cell imaging of annexin V and PI-labeled cells, a microscope cage incubator with dark panels (Okolab, Naples, Italy) was pre-warmed and maintained at 37 °C during the imaging. An H201temperature unit (Okolab) was used to control the temperature. Live-cell imaging was performed in Hibernate E medium containing 2% B-27 Plus and 1% PS.
Live-cell imaging of neurons expressing NFL-GFP and NFL(ΔA461-D543)-GFP was performed by using the incubator and the heating unit described above. The incubator was pre-warmed to 37 °C and neurons in artificial cerebro-spinal fluid (aCSF) containing 2% B-27 Plus and 1% PS were placed on the stage. In each well, 10 neurons expressing either NFL-GFP or NFL(ΔA461-D543)-GFP were selected, and the xyz coordinates of each field of view were saved in NIS-Elements AR software. After the acquisition of the first set of images, NONOate solutions were prepared in aCSF (containing 2% B-27 Plus and 1% PS), to a double concentration of 1 mM. Diluted NONOates were added to wells at a 1:1 ratio with the volume of medium already present to achieve a final concentration of 0.5 mM. Images were acquired after the addition of the NONOate, and then every 10 min until approximately 1 h after treatment began.
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