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Polycarbonate 12 well transwell inserts

Manufactured by Corning
Sourced in United States

Polycarbonate 12-well transwell inserts are a laboratory equipment product used for cell culture experiments. They provide a platform for studying cell migration, invasion, and permeability. The inserts are made of polycarbonate material and feature 12 individual wells arranged in a multiwell plate format.

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2 protocols using polycarbonate 12 well transwell inserts

1

Sodium Fluorescein Permeability Assay

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Sodium fluorescein-flux assays were conducted as previously described (28 (link)). Caco2 cells were plated on collagen I coated polycarbonate 12-well transwell inserts (0.4 μm pore size, Corning) and allowed to reach confluence. The luminal (upper) compartment was treated with sodium fluorescein (2.5 mg/mL) for 15 minutes, then 100 μL aliquots were obtained from each abluminal (lower) compartment and assayed for fluorescence intensity. Permeability coefficients (Ps) were calculated using the formula Ps=[Ab]/t× 1/A×V/[Lu], where [Ab] is the abluminal concentration of sodium fluorescein, t is time in seconds for sodium fluorescein incubation, A is area of membrane in cm2, V is the volume of the abluminal chamber, and [Lu] is the luminal concentration of sodium fluorescein. Results are representative of 4 experiments *p<0.05.
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2

In Vitro Sodium Fluorescein Permeability Assay

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Briefly, bEnd.3 cells were seeded onto polycarbonate 12-well transwell inserts with a 0.4-μm mean pore size and a 0.33-cm2 surface area (Corning, USA) at a density of 4 × 104 cells/cm2, and the growth medium was refreshed every other day. The seeded cells were allowed to grow at 37 °C in a 5% CO2/95% air atmosphere until they reached 70–80% confluence, which was confirmed using phase contrast microscopy. Then, cells were cultured with different ACMs for 24 h. After two washes with PBS, the media in the transwell inserts were replaced with media supplemented with 500 μL of 1 mg/mL sodium fluorescein (NaF), the lower chamber was filled with 1000 μL of normal media, and cells cultured for 1 h at 37 °C under normoxic conditions. Relative fluorescence passing through the chamber was measured as follows: 100 μL of medium in the lower chamber was assayed in triplicate in black 96-well plates (Corning, USA). The fluorescence intensity was measured using an EnSpire Manager (PerkinElmer, USA) multimode plate reader at an excitation wavelength of 460 nm and an emission wavelength of 515 nm [11 (link)]. NaF permeability (μg/cm2) = total NaF quantity in the lower chamber/the surface area of insert (0.33 cm2).
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