Реакция #57129
ord-58a14e020d284bcb82a1da0fb03517d5
Уравнение реакции
Условия реакции
Обработка
- 1workup.WAITOn day 1, cells were plated at 3,000 cells
- 2workup.ADDITIONPlates containing cells with 200 μl of assay
- 3workup.ADDITIONto addition of compounds
- 4workup.ADDITIONcontaining cells for a final tert concentration of 1 μM
- 5workup.ADDITIONdiluted in assay
- 6workup.ADDITIONTwenty-five microliters of assay buffer (maximum NE uptake) or tert compound were added directly
- 7workup.ADDITIONcontaining cells in 200 μl of assay buffer
- 8workup.WAITThe cells in assay buffer with tert compounds were incubated for 20 minutes at 37° C
- 9workup.ADDITIONdiluted in assay buffer (120 nM final
- 10Концентрированиеassay concentration)
- 11workup.WAITthe plates were incubated for 5 minutes
- 12Другое(37° C.)
- 13ДругоеThe reaction was terminated
- 14Другоеby decanting the supernatant from the plate
- 15workup.ADDITIONThe plates containing cells
- 16Промывкаwere washed twice with 200 μl assay buffer (37° C.)
- 17Другоеto remove free radioligand
- 18workup.WAITleft
- 19Другоеto dry for 2 minutes
- 20Другоеair-dried for an additional 10 minutes
- 21Другоеwere lysed in 25 μl of 0.25 N NaOH solution (4° C.)
- 22workup.ADDITIONAfter cell lysis, 75 μl of scintillation cocktail was added to each well
- 23Другоеthe plates were sealed with film tape
- 24workup.STIRRINGvigorously shaken for a minimum of 10 minutes
- 25Другоеto ensure adequate partitioning of organic and aqueous solutions
- 26Другоеto collect the raw cpm data
Методика
On day 1, cells were plated at 3,000 cells/well in growth medium and maintained in a cell incubator (37° C., 5% CO2). On day 2, growth medium was replaced with 200 μl of assay buffer (25 mM HEPES; 120 mM NaCl; 5 mM KCl; 2.5 mM CaCl2; 1.2 mM MgSO4; 2 mg/ml glucose (pH 7.4, 37° C.)) containing 0.2 mg/ml ascorbic acid and 10 μM pargyline. Plates containing cells with 200 μl of assay buffer were equilibrated for 10 minutes at 37° C. prior to addition of compounds. A stock solution of desipramine was prepared in DMSO (10 mM) and delivered to triplicate wells containing cells for a final tert concentration of 1 μM. Data from these wells were used to define non-specific NE uptake (minimum NE uptake). Test compounds were prepared in DMSO (10 mM) and diluted in assay buffer according to tert range (1 to 10,000 nM). Twenty-five microliters of assay buffer (maximum NE uptake) or tert compound were added directly to triplicate wells containing cells in 200 μl of assay buffer. The cells in assay buffer with tert compounds were incubated for 20 minutes at 37° C. To initiate the NE uptake, [3H]NE diluted in assay buffer (120 nM final assay concentration) was delivered in 25 μl aliquots to each well and the plates were incubated for 5 minutes (37° C.). The reaction was terminated by decanting the supernatant from the plate. The plates containing cells were washed twice with 200 μl assay buffer (37° C.) to remove free radioligand. The plates were then inverted, left to dry for 2 minutes, then reinverted and air-dried for an additional 10 minutes. The cells were lysed in 25 μl of 0.25 N NaOH solution (4° C.), placed on a shake table and vigorously shaken for 5 minutes. After cell lysis, 75 μl of scintillation cocktail was added to each well and the plates were sealed with film tape. The plates were returned to the shake table and vigorously shaken for a minimum of 10 minutes to ensure adequate partitioning of organic and aqueous solutions. The plates were counted in a Wallac Microbeta counter (PerkinElmer) to collect the raw cpm data.