NOTE: There is a methods document PDF version of this information included as a supplementary file.
PROCEDURE
Preparation
1. Warm cell culture media and DPBS in a 37 °C water bath (hereafter referred to as “warmed” medium or DPBS).
2. Ensure that the EVOM2 unit is fully charged.
NOTE: If unsure, leave the EVOM2 unit plugged into an electrical outlet for 30 minutes before beginning your TEER assay.
NOTE: According to the manufacturer, taking TEER measurements while the EVOM2 unit is plugged into an electrical outlet can increase variability in your samples.
3. Acquire an additional 12-well plate (“holding plate”) before starting any measurement.
a. A subset of your sample inserts will be held in this plate before transfer to the EndOhm-12 cup chamber.
4. Adjust the probe height on the EndOhm-12 unit (when applicable).
a. A manufacturer provided EndOhm-12 unit spacer can be used to reset the probe height on the EndOhm-12 cap probe to the factory standard.
b. Place a blank insert into the EndOhm-12 cup chamber, and the spacer inside the blank insert.
c. Loosen the locking nut on the cap probe and rotate the cap to change the height of the electrode until it touches the spacer.
d. For experimental applications, the cap probe electrode should be adjusted to be submerged in apical medium.
5. Clean the EndOhm-12 by rinsing the cap and chamber with distilled water, then alcohol, then distilled water again and allow to dry before reassembling.
6. Clean the working surface of the biosafety cabinet (BSC) with Cavicide, then spray the working surface with 70% ethanol and wipe with paper towel(s).
a. Allow surface to air dry before putting materials into the BSC.
Measuring blank resistance
1. Place the EndOhm-12 cup chamber and the holding plate into a cleaned BSC.
2. Add 3.0 mL of warmed cell culture media to the EndOhm-12 cup chamber using a 5 mL serological pipet.
3. Place the blank insert into the holding plate and add 500 μL of cell culture media to the apical compartment using a P1000 pipette.
4. Transfer the blank insert into the EndOhm-12 cup chamber.
a. Check for bubbles underneath the blank insert.
b. Remove the insert and transfer the insert back into the EndOhm-12 cup to remove any bubbles.
c. Placing the insert into the EndOhm-12 cup at an angle can reduce the frequency of bubbles.
5. Plug the EVOM2 connecting wires into the EndOhm-12 cup chamber, place the EndOhm-12 into a cell culture incubator, and close the door (Figure 1).
6. Switch the EVOM2 on.
a. The blank resistance readings should stabilize within a few seconds.
7. Switch the EVOM2 off and return the EndOhm-12 to the BSC.
8. Transfer the blank insert back to the holding plate.
Measuring sample resistance
1. Remove samples from the cell culture incubator and transfer to a BSC.
2. Transfer your first three Transwell inserts to be assayed to the holding plate.
a. Transferring three samples to the holding plate at a time allows the remaining samples to be returned to the climate-controlled environment of the cell culture incubator.
3. If medium is present in the apical compartment of the Transwell inserts in the holding plate then remove it by aspiration.
4. Rinse inserts in the holding plate with 500 μL of warmed DPBS using a P1000 pipette.
5. Add 500 μL of warmed cell culture media to your sample inserts using a P1000 pipette.
6. Transfer your sample insert into the EndOhm-12 cup chamber.
a. Check for bubbles underneath the blank insert.
b. Remove the insert and transfer the insert back into the EndOhm-12 cup to remove any bubbles.
c. Placing the insert into the EndOhm-12 cup at an angle can reduce the frequency of bubbles.
7. Plug the EVOM2 connecting wires into the EndOhm-12 cup chamber, place the EndOhm-12 into a cell culture incubator, and close the door (Figure 1).
8. Switch the EVOM2 on.
a. Resistance readings should stabilize within 5 minutes.
b. Resistance stabilization time is cell type and cell condition dependent.
9. Switch the EVOM2 off and return the EndOhm-12 to the BSC.
10. Exchange sample inserts and repeat steps 7-9.
11. Return the sample insert set from the Holding Plate to the original Sample Plate.
a. Repeat steps 2-9 with the remaining samples.
Clean up
1. Return the EVOM2 unit to its box.
2. Aspirate all media out of the EndOhm-12 cup chamber.
3. Rinse both the EndOhm-12 cup chamber and the EndOhm-12 cap probe with ddH2O, spray with 70% Ethanol, and rinse one final time with ddH2O.
a. Ensure no water floods the electronic connection ports.
4. Allow the EndOhm-12 cup chamber to air dry.
5. Return the EndOhm-12 Unit to its bubble wrap and storage box.
Data analysis
1. TEER values are expressed as W cm2, which can be determined by multiplying the resistance values obtained above (in W) by the surface area of the insert in cm2 (Corning 12 mm insert surface area = 1.12 cm2).
2. Determine the mean TEER of the blank samples and subtract this value from all of the sample TEER values.
3. TEER data and differences/changes in TEER should be reported as actual TEER values (using the units of W cm2) and not fold or percent changes.
QUALITY CONTROL RATIONALE
If the equipment is not cared for or calibrated it will result in incorrect readings. Use the provided test resistor to test the EVOM prior to each round of data collection. The test resistor is 1000 W. If test resistor does not read 1000 W then use a screwdriver to adjust the EVOM unit in the R ADJ port.