The HTRF Total IKZF3 assay quantifies the expression level of IKZF3 in a cell lysate. Unlike Western Blot, the assay is entirely plate-based, and does not require gels, electrophoresis, or transfer. The Total IKZF3 assay uses two labeled antibodies, one coupled to a donor fluorophore and the other to an acceptor. Both antibodies are highly specific for a distinct epitope on the protein. In presence of IKZF3 in a cell extract, the addition of these conjugates brings the donor fluorophore into close proximity with the acceptor, and thereby generates a FRET signal. Its intensity is directly proportional to the concentration of the protein present in the sample, and provides a means of assessing the protein’s expression under a no-wash assay format.

The 2-plate protocol involves culturing cells in a 96-well plate before lysis, then transferring lysates into a 384-well low volume detection plate before the addition of the Total IKZF3 HTRF detection reagents. This protocol enables the cells' viability and confluence to be monitored.

Detection of Total IKZF3 with HTRF reagents can be performed in a single plate used for culturing, stimulation, and lysis. No washing steps are required. This HTS-designed protocol enables miniaturization while maintaining robust HTRF quality.

Ramos cells were seeded in 96-well culture plate (50,000 cells/30µL well) and treated with increasing concentrations of the CELMoD  Avadomide for 4h or 24h. The proteasome inhibitor epoxomicin (1µM) was added or not 1h prior to the addition of Avadomide .

After treatment, cells were lysed with 10 µl of supplemented lysis buffer #4 (4X) for 30 min at RT under gentle shaking. Next, 16 µL of lysate were transferred into a 384-well low volume white microplate, and 4 µL of the HTRF Total IKZF3 detection antibodies were added. An additional 4 µL of lysate (supplemented with 12 µL diluent #8) were also transferred into the microplate to check the alpha-tubulin level with the alpha-tubulin housekeeping Cellular Kit (64ATUBPET/G/H). HTRF signals were recorded after an overnight incubation.

The CELMoD Avadomide induced a dose-dependent decrease in IKZF3 protein levels, with DC₅₀* of 56 nM and 29 nM after 4h and 24h respectively. Furthermore, Avadomide-induced IKZF3 degradation was prevented in the presence of epoxomicin, a proteasome activity inhibitor. This result unambiguously demonstrates that Avadomide-induced IKZF3 degradation is mediated by the ubiquitin proteasome system. Similar data were obtained when treating cells with Lenalidomide (IMID) or Iberdomide (CELMoD) (data not shown).

* DC₅₀  corresponds to the concentration of the degrader at which 50% of the targeted protein is degraded.

HAP1 cells were transfected with human IKZF3, human IKZF1 plasmids in a T175 flask and incubated for 24h. After medium removal, cells were lysed with 3 mL of supplemented lysis buffer #4 (1X) for 30 min at RT under gentle shaking.

The IKZF3 expression levels were assessed with the HTRF Total IKZF3 kit. Briefly, 16 µL of cell lysate were transferred into a low volume white microplate, followed by 4 µL of premixed HTRF detection reagents. The HTRF signal was recorded after an overnight incubation at RT.

The HTRF Total IKZF3 assay efficiently detected IKZF3 in the IKZF3 transfected HAP1 cells compared to the WT HAP1 cells. No signal was detected in IKZF1 transfected cells, demonstrating the specificity and selectivity of the kit.

The suspension cell lines MOLT-4 (T lymphoblast), Ramos (B lymphocyte), and Raji (B lymphoblastoid) were dispensed into a 96-well plate, and lysed with 10 µL of supplemented lysis buffer #4 (4X) for 30 min at RT under gentle shaking (performed according to the suspension cell protocol).

The IKZF3 expression level was assessed with the HTRF Total IKZF3 kit. Briefly, 16 µL of cell lysate were transferred into a low volume white microplate, followed by 4 µL of premixed HTRF detection reagents. The HTRF signal was recorded after an overnight incubation at RT. The dotted line corresponds to the non-specific HTRF signal. Note that the cell density was optimized beforehand to ensure HTRF detection within the dynamic range of the kit (data are shown for 100,000 cells/well)

The HTRF Total IKZF3 assay efficiently detected endogenous IKZF3 in various cellular models expressing different levels of the protein.

Ramos cells were cultured in a T175 flask in complete medium at 37°C, 5% CO2. After medium removal, the cells were lysed with 3 mL of supplemented lysis buffer #4 (1X) for 30 min at RT under gentle shaking.

Serial dilutions of the cell lysate were performed using supplemented lysis buffer #4 (1X), and 16µL of each dilution were transferred into a 384-well small volume microplate before the addition of 4µL of HTRF Total IKZF3 detection antibodies. HTRF signals were recorded after an overnight incubation.

Equal amounts of lysates were loaded into a gel for a side-by-side comparison between HTRF and Western Blot.

In these conditions, the HTRF Total IKZF3 assay is 16-fold more sensitive than the Western Blot technique.

Ikaros zinc finger transcription factors are important regulators of the gene programs underlying the development of hematopoietic cell lineages. They recruit different co-factors and interact with target gene loci or chromatin-remodeling complexes. Ikaros mediate different transcriptional outcomes by acting as transcriptional repressors or activators based on cell type.