Quantitative, Real-Time Measurements of Intracellular Target Engagement Using Energy Transfer

3.1.1 Example Synthesis of Amine-Linked Tracers:

Charge the small molecule precursor, functionalized with an amine, (9.9micromolar (µM)) into a 5 mL amber vial.

Dry the resulting film for a minimum of 1h 0m 0s to remove trace volatile solvents.

Dissolve the resulting solid in an appropriate volume of DMSO to give a 2.0millimolar (mM) solution.

Calculate the concentration of the solution using the following molar extinction coefficients:

ε_NanoBRET™

₅₉₀ = 83,000 M⁻¹ cm⁻¹, ε_NanoBRET™

₆₁₈ = 96,000 M⁻¹ cm⁻¹.

Add 0.5mL and stir.

Add 8.6µL, allowing the mixture to stir for 0h 10m 0s.

Add 5mg. Cap and allow to react in the dark for 1h 0m 0s.

Monitor the reaction for consumption of the starting amine by analytical HPLC. The reaction is judged complete when this material has been consumed. The reaction progresses quickly and is often near completion after 0h 30m 0s( see   Note 1 ).

Dilute the crude mixture with the reaction quenching solution.

Purify the compound using reverse-phase preparative HPLC. Most tracers can be purified using standard HPLC methods. Use a gradient of trifluoroacetic acid (TFA) HPLC Buffer (or 0.1% formic acid in water) in acetonitrile as an eluent.

Pool product containing fractions and concentrate to dryness under reduced pressure.

Dissolve the resulting film in approximately 10mL and concentrate to dryness a total of three times ( see   Note 2 ).

Cultivate desired cells (e.g., HEK293) appropriately prior to assay and resuspend cells into a single-cell suspension using complete cell culture medium.

Adjust the cell density to 2 × 10⁵/mL in cell culture medium in a sterile, conical tube.

Prepare plasmid DNAs for transfection. For first-time experiments, use a 1:10 dilution (mass:mass) of expression construct into a promoterless DNA (Transfection Carrier DNA). At this stage it may be useful to perform a titration of expression, by diluting the expression construct into Transfection Carrier DNA. Examples of extending this titration are shown in Fig. 6.

Prepare transfection complexes using the manufacturer’s protocol.

Mix one part (e.g., 1 mL) of transfection complex with 20 parts (e.g., 20 mL) of HEK293 cells in suspension at 2 × 10⁵/mL. Mix gently by inversion five times in a sterile, conical tube.

Dispense cells/lipid–DNA complex into a sterile tissue culture flask, and incubate at least 20h 0m 0s to allow expression to occur. We recommend a cell density of approximately 55,000–80,000 cells/cm² during the transfection (for example use approximately 4−6 million cells for a T75 flask). Larger or smaller bulk transfection should be scaled accordingly, using this ratio.

Harvest cells via trypsinization, and resuspend in growth medium including serum. Centrifuge the cells and resuspend the pellet in Opti-MEM without serum or phenol red.

Adjust the cell density to 2 × 10⁵/mL in Opti-MEM without serum or phenol red.

Prepare cells for target engagement analysis in live or permeabilized cells. For live cell target engagement experiments, dispense 85µL per well into white, 96-well NBS plate. Periodically mix cells appropriately to avoid settling of the cell suspension. For live cell analysis, proceed to  step 13 . For permeabilized cell experiments dispense 68µL per well into a white, 96-well plate. Add 17µL (either 5× Passive Lysis Buffer or 250 μg/mL digitonin).

Prepare the complete 20× tracer. For characterization of tracer affinity, perform a serial dilution of the tracer in DMSO at a 100× concentration ( see   Note 4 ). For characterization of unlabeled drug affinity (if the optimal concentration of tracer has already been determined) prepare a 100× concentration of the tracer in pure DMSO.

Dilute the 100× tracers to 20× with Tracer Dilution Buffer according to the manufacturer’s instructions. Add 4 parts Tracer Dilution Buffer to 1 part of 100× tracer (from DMSO) to prepare the Complete 20× tracer reagent.

Mix gently several times to ensure that the DMSO solution is mixed with the tracer dilution buffer.

Add 5µL per well to cells in suspension.

Mix on orbital shaker for 0h 0m 15s at 900rpm. Mixing may vary between orbital shakers and should be optimized for each individual unit accordingly. Due to the viscosity of the Tracer Dilution Buffer, it is necessary to dispense this solution slowly.

Prepare a suitable unlabeled test compound at 1000× final concentration in 100% DMSO. Typically, the 1000× concentration of compound is in the 10millimolar (mM)–100millimolar (mM) range. Then dilute to a 10× final concentration in Opti-MEM without serum or phenol red.

The characterization of BRET tracers can be performed as a single concentration of unlabeled compound for tracer dose–response curves. It is generally recommended that a 20−100× molar excess of parental drug is coincubated with the tracer to determine the nonspecific BRET signal.

For characterization of unlabeled drug IC₅₀, create a serial dilution of test compound for drug IC₅₀ analysis.

Add 10µL per well to the 96-well plates containing cells with 1× tracer. Mix on orbital shaker for 0h 0m 15s at 900rpm.

Incubate the plate at 37°C and 5% CO2 for 2h 0m 0s. Allow plate to cool to Room temperature for approximately 0h 15m 0s, then proceed to the next section below. (step 24)

For permeabilized cell assays, incubate the plate at Room temperature, protected from light for 1h 0m 0s−2h 0m 0s(depending on the characteristics of the test compound). Then proceed with the next step ( see  Section 3.2.4 "Detection in Microplate Luminometer Equipped with Appropriate BRET Filters").

Immediately prior to BRET measurements, prepare 3× Complete NanoBRET(TM) Nano-Glo(R) Substrate.

For live cell analysis, add Extracellular NanoLuc(R) Inhibitor in Opti-MEM and add to cells according to the manufacturer’s instructions (Promega) ( see   Note 5 ).

For Permeabilized cell analysis, prepare 3× NanoBRET(TM) Nano-Glo(R) Substrate in Opti-MEM without serum or phenol red, and omit the Extracellular NanoLuc(R) Inhibitor. This solution consists of only a 1:166 dilution of NanoBRET(TM) Nano-Glo(R) Substrate in Opti-MEM.

Following addition of 50µL, measure donor emission (e.g., 450 nm) and acceptor emission (e.g., 610 nm or 630 nm) using a NanoBRET(TM)-compatible luminometer.

To generate raw BRET ratio values, divide the acceptor emission value (e.g., 610 nm) by the donor emission value (e.g., 450 nm) for each sample. Convert raw BRET units to milliBRET units (mBU) by multiplying each raw BRET value by 1000.

(Optional) If a background correction is desired, use the NanoBRET Equation (Eq. 1).

(1)

Aliquot test and control compound stocks in 100% DMSO at high concentration (typically either 5millimolar (mM) or 10millimolar (mM) depending on desired final assay concentration of 10micromolar (µM) or 20micromolar (µM), respectively) to acoustic dispense qualified mother plates. Depending on equipment, one or more additional dilutions likely are required.

Adjust instrument to dispense 80 nL of highest concentration, then 1:3 dilutions using 100% DMSO as backfill in order to create a 12-point dilution series of 80 nL total volume in each well. Since the lowest dispense amount may be 5 nL, several intermediate dilutions of the initial 5 or 10 mM stock likely are required to achieve the required dispenses.

Seal plates tightly and store at 4°C until day 2 of assay.

Harvest cells as described in Section 3.2.2 "[Day 2]: Preparation of Cells with 1× Tracer for BRET Assay" and adjust the cell density to 2 × 10⁵/mL in Opti-MEM without serum or phenol red.

Dispense 38µL per well into white, 384-well plate containing previously dispensed, serially diluted test and control compounds.

Prepare the BRET tracer at the lowest concentration determined to yield a useable signal:background and Z’ greater than 0.5, optimally 50−80% of full target occupancy.

Add 2µL per well to cells in suspension. Mix thoroughly using appropriate instrumentation.

Incubate plates in a humidified, 37°C/5% CO2 incubator for 2h 0m 0s.

Add 20µL per well for a 384-well plate. Incubate 0h 2m 0s–0h 3m 0s at Room temperature prior to first read; readings are stable at least 1h 0m 0s.

Measure BRET as described in Section 3.2.4 "Detection in Microplate Luminometer Equipped with Appropriate BRET Filters."

After transfecting cells (as described in Section 3.2.1 "[Day 1]: Transient Transfection of HEK293 Cells with NanoLuc(R) Fusions"), resuspend cells using prewarmed assay medium (e.g., Opti-MEM without serum or phenol red).

Adjust the density to 2 × 10⁵ cells/mL in assay medium in a 15 mL sterile polypropylene conical tube. We recommend a minimum volume of 1 mL of cells, ideally 5 mL of cells.

Prepare test compound at 10× final concentration in appropriate solvent (e.g., 1% DMSO).

To determine the optimal concentration of test compound for residence time analysis, it is recommended to first determine the compound IC₅₀ using the equilibrium-based Target Engagement Protocol (see Section 3.2.2 "[Day 2]: Preparation of Cells with 1× Tracer for BRET Assay"). Introduce the test compound at a final concentration of 10–20×  K _i,app determined under equilibrium conditions. This insures that adequate washout conditions can be achieved prior to off-rate measurements. Add 100µL to each 1 mL of cells in assay medium and mix gently.

(Optional) Include a positive control treatment of a compound at a high and saturating dose as a full-occupancy control, as well as a negative control treatment with compound vehicle.

Place the conical tube in a rack, and incubate the tube with the cap loosened at 37°C, 5% CO2 for a minimum of 2h 0m 0s or until sample is expected to reach equilibrium.

To prepare Complete 20× tracer reagent, first prepare a 100× solution of BRET tracer in 100% DMSO. Add 4 parts Tracer Dilution Buffer to 1 part of 100× tracer to generate Complete 20× tracer reagent.

For analysis of residence time in live cells, prepare a 2× solution of NanoBRET(TM) Nano-Glo(R) Substrate plus Extracellular NanoLuc Inhibitor by diluting the NanoBRET(TM) Nano-Glo(R) Substrate 1:250 and the Extracellular NanoLuc(R) Inhibitor 1:750 in a conical tube with Opti-MEM without serum or phenol red.

For example:

For a 96-well plate, mix 40µL, 13.3µL, and 9946µL to produce 10 mL of 2× NanoBRET™ Nano-Glo(R) Substrate plus Extracellular NanoLuc(R) Inhibitor Solution.

Mix gently by inversion 5–10 times.

For analysis of residence time in permeabilized cells, include 100 μg/mL digitonin and omit the Extracellular NanoLuc(R) inhibitor in the 2× solution.

After incubation with test compound is complete, centrifuge cells at 200x g.

Optional Wash: To remove unbound test compound, resuspend cells in prewarmed assay medium, centrifuge cells and remove medium. Maintain the concentration of the positive control compound for the full-occupancy control.

Remove medium, resuspend cells in prewarmed assay medium, and adjust cell density to 2 × 10⁵ cells/mL.

Dispense 90µL per well into white, 96-well plates. Periodically mix cells to avoid cell settling in the tube.

(Optional) For background correction, dispense 100µL in triplicate as no-tracer control samples.

Add 100µL prepared above (see Section 3.5.2 "Preparing BRET Reagents").

Dispense 10µL per well to cells. Mix the 96-well plate on an orbital shaker for 900rpm.

(Optional) Prepare a separate set of samples without tracer for optional background correction steps.

Immediately proceed to the next step (see Section 3.5.4 "BRET Detection in Kinetic Mode").

Set a NanoBRET™ Assay-compatible instrument to perform repeat measurements for the desired time interval. As a starting point, use 0h 5m 0s intervals between each measurement, and be sure to include a sufficient number of measurements to determine compound dissociation. Set the instrument at 25°C to minimize sample evaporation. However, as temperature may impact residence time profiles, it may be valuable to evaluate physiological temperatures.

Measure donor emission wavelength (e.g., 450 nm) and acceptor emission wavelength (e.g., 600 nm), and determine the BRET ratio as described earlier (see Section 3.2.4 "Detection in Microplate Luminometer Equipped with Appropriate BRET Filters").

Mix desired cells with lipid–DNA complexes as described in Section 3.2.1 "[Day 1]: Transient Transfection of HEK293 Cells with NanoLuc(R) Fusions".

Dispense 100µL into a sterile, tissue-culture treated 96-well plate, and incubate at least 20h 0m 0s to allow expression. We recommend a cell density of approximately 55,000–80,000 cells/cm² during the transfection (for example, use approximately 20,000 cells/well for a 96-well Corning #3917 assay plate).

On day 2, gently remove medium from the assay plate with transfected HEK293 cells via aspiration.

Add back 90µL per well. Include suitable controls as indicated in Sections 3.5.1 "Adding Test Compound to Cells" and 3.5.3 "Preparing Cells and Dispensing Reagents for the Residence Time Assay."

Add 10µL to each assay well. For full-occupancy control, include a sample with a saturating dose of a positive control compound. For zero-occupancy control, add only DMSO. If the optional “No tracer control samples” were added to the experiment, do not add test compound.

Mix on orbital shaker for 900rpm.

Incubate the assay plate at 37°C, 5% CO₂ for a minimum of 2h 0m 0s or until sample is expected to reach equilibrium. Shorter or longer incubation times may be required depending on the characteristic of the test compound.

After incubation with test compound is complete, gently aspirate to remove the medium and test compound from the assay plate. For the full-occupancy control, do not perform this step. Test compound should remain in the sample.

To remove residual unbound test compound, gently add 150µL to each well and incubate at Room temperature for 0h 0m 30s. For the full-occupancy control, do not perform this step. Test compound should remain in the sample.

Gently aspirate the medium and dispense 90µL per well.

Add 100µL to each well of the 96-well plate (prepared as described in Section 3.5.2 "Preparing BRET Reagents" in the protocol for residence time in NBS format).

Dispense 10µL per well. Mix the 96-well plate on an orbital shaker for 900rpm.

Immediately measure BRET in kinetic mode as described in Section 3.5.4 "BRET Detection in Kinetic Mode" in the protocol for residence time in NBS format.

Process data as described above in the protocol for residence time in NBS format (see Section 3.5.4 "BRET Detection in Kinetic Mode").