Transcription Factor Activity Assay Sample Protocol

The ELISA Genie Transcription Factor Activity Assay Kit allows for the detection and qualitative analysis of endogenous levels of activated transcription factors (e.g. NF-κB, p53, SMAD) in a variety of nuclear and cell lysates. The ease-of-use of our assays mean that runtime is significantly shorter than common methods of detection of transcription factors. Below are the preparation steps for the assay, storage guidelines, and protocols for both nuclear and cytoplasmic extraction, as well as the Transcription Factor Activity ELISA protocol itself.

The following reagents will need to be prepared prior to start of the assay:

The Wash Buffer is provided at 10x concentration. To prepare 1x Wash Buffer, add 50 ml of 10x Wash Buffer into 450 ml of ddH2O for a final volume of 500 ml of 1x Wash Buffer.

The Binding Buffer is provided at 2x concentration. It is recommended to make fresh 1x Binding Buffer for the reconstitution of Nuclear Lysate Positive Control. Add 60 µl of 2x Binding Buffer to 60 μl ddH2O to make 120 μl of 1x Binding Buffer. Add 100 μl of 1x Binding Buffer into the Nuclear Lysate Positive Control tube. The Nuclear Lysate Positive Control should be kept on ice at all times. Aliquot and store at -80°C (long term storage) and avoid freeze/thaw cycles if not immediately used.

The Primary Antibody and/or Primary Phospho-Antibody is provided at 100x concentration. It is recommended to make fresh 1x Primary Antibody solutions. Add 100 μl of 100x Primary Antibody or Primary Phospho-Antibody into 9.9 ml of Primary Antibody Diluent to make enough 1x Primary Antibody or 1x Primary Phospho-Antibody solution for one 96-well microplate.

If you do not plan on using the whole kit in one sitting, it is recommended to aliquot the:

• Buffers and reagents
• Reconstituted Nuclear Lysate Positive Control
• 2x Binding Buffer
• Cytoplasmic Extraction Buffer
• Nuclear Wash Buffer
• Nuclear Extraction Buffer, etc.

and store them at the temperatures indicated in the table on page 7 of each individuals kit techincal manual.

The following reagents are ready-to-use:

• HRP-Conjugated Anti-Rabbit IgG Secondary Antibody
• Ready-to-Use Substrate
• Stop Solution
• Primary Antibody Diluent
• Wild-Type (WT) Consensus dsDNA Oligonucleotide
• Mutant (MT) Consensus dsDNA Oligonucleotide
• Nuclear Wash Buffer
• Cytoplasmic Extraction Buffer
• Nuclear Extraction Buffer
• Stablization Buffer
• Termination

The following materials and/or equipment are NOT provided in this kit but are necessary to successfully conduct the experiment:

• Microplate reader able to measure absorbance at 450 nm (with correction wavelength set to 540 nm or 570 nm)
• Micropipettes capable of measuring volumes from 1 μl to 1 ml
• Deionized or sterile water (ddH2O)
• PMSF (Sigma Cat. #78830)
• Protease Inhibitor Cocktail (Sigma Cat. # P-2714)
• Glycerol (Acros Cat. #158920100)
• Sterile 1x PBS and 5 M NaCl for nuclear lysate preparation
• Squirt bottle, manifold dispenser, multichannel pipette reservoir, or automated microplate washer
• Graph paper or computer software capable of generating or displaying logarithmic functions
• Absorbent paper or vacuum aspirator
• Test tubes or microfuge tubes capable of storing ≥1 ml
• Bench-top centrifuge (optional)
• Bench-top vortex (optional)
• Orbital shaker (optional)

All preparations of experimental samples within the ELISA Genie Transcription Factor Activity Assay Kit should maintain the natural and active form of the target transcription factor. In this kit, not all buffers and reagents are provided for nuclear extraction from cell culture.

Tissue homogenates and heterogeneous mixtures may contain contaminants which interfere with the assay, hence it is best to test for interference by using at least two different dilutions of the sample. If testing demonstrates good correlation between concentration/dilution factor and OD reading, purification may not be required. However, if good correlation is not achieved or seen, further purification is advised. Moreover, if samples contain any visible precipitate, they must be centrifuged for 10 minutes at ≥10,000 x g prior to use in the assay.

It is always recommended to make several dilutions to obtain the best OD reading. Ideal OD readings will fall within the detectable range of the assay, which is dependent on the spectrophotometer used. It is up to the investigator to determine an appropriate dilution factor and recommended to run each dilution in duplicates. A minimum of 100 µl of sample or diluted sample is required for each well; please adjust dilution volumes accordingly.

If samples are ready to be used within 24 hours, aliquot and store at 4°C. If samples are to be saved for future or long term use, aliquot into multiple tubes and store at -80°C. Avoid repeated freeze/thaw cycles to prevent loss of biological activity of transcription factors in experimental samples. If a sample contains any visible precipitate or pellet, it must be clarified prior to use in the assay.

The ELISA Genie Transcription Factor Activity Assay kit includes some of the necessary buffers for nuclear and cytoplasmic extraction from cultured cells. These buffers must be supplemented with PMSF (not included) and Protease Inhibitor Cocktail (no included) immediately prior to use. For the Protease Inhibitory Cocktail, we recommend one from Sigma-Aldrich (Cat. # P-2714).

Many transcription factors may not be readily expressed in normal cell culture, therefore cell stimulation is often needed to increase the expression of target protein. Use this protocol for cytoplasmic and nuclear extraction following your own cell stimulation/cell culture protocol.

The PMSF Stock Solution, Inhibitor PBS Buffer, Complete Cytoplasmic Extraction Buffer, and the Complete Nuclear Extraction Buffer should all be prepared prior to extraction. PMSF is unstable and must be added fresh just prior to use. Buffers with protease/phophatase added in, like PMSF, has a 24- hour shelf-life at 4°C.

Note: This is just a recommended protocol for your convenience. You may need to optimize the cell extraction procedure for your own experiments and applications.

Materials: PMSF, DMSO, 1.5ml microfuge tube

Materials: 1x PBS, PMSF Stock Solution (100mM), Protease Inhibitor Cocktail

Materials: Cytoplasmic Extraction Buffer, PMSF Stock Solution (100mM), Protease Inhibitor Cocktail

Materials: Nuclear Extraction Buffer, PMSF Stock Solution (100mM), Protease Inhibitor Cocktail

The 96-well microplate provided with this kit is ready to use and coated with streptavidin bound to biotinylated oligonucleotides, which will allow activated transcription factor binding. It is not necessary to rinse plates prior to assay. It is recommended to assay all unknown samples and controls in duplicates. If not all the strips are used at once, keep unused strips sealed and store at 4°C.

A number of controls are included to ensure kit and data quality. It is recommended to run the Nuclear Lysate Positive Control (NLPC) as well as to perform a Primary Antibody negative control to determine background noise. The Wild-Type Consensus dsDNA Oligonucleotide (WT Oligo) and Mutant Consensus dsDNA Oligonucleotide (MT Oligo) controls are optional and used to determine binding specificity of activated transcription factors in samples.

The following is an example of a setup that can be used.

If possible, all incubation steps should be performed on an orbital shaker to allow added solutions to equilibrate and mix properly. Aside from the Nuclear Lysate Positive Control, all provided solutions should be brought to ambient temperature prior to use.

Ensure all 1x Wash Buffer is removed at end of each wash step by blotting a dry towel. DO NOT leave any 1x Wash Buffer in the wells prior to proceeding to the next steps as it may affect assay results.

The Wild-Type Oligonucleotide and Mutant Oligonucleotide controls are optional and used to determine binding specificity of active transcription factors in samples. If active transcription factors in samples are binding specifically to the Wild-Type sequence, there will be a reduction in signal in the Wild-Type control but not in the Mutant control. If they are binding non-specifically, there will be reduced signal from both Wild-Type and Mutant Oligonucleotide controls.

Transcription Factors are expressed differently across various tissues, cell types, growth stages, and culture conditions. Carefully determine the amount of sample used; we recommend 5 μg or more of cell lysate per well. If the sample concentrations are unknown, create several dilutions. It is recommended to perform a Primary Antibody negative control for sample wells to determine background noise. It is also recommended to run your samples in duplicates or triplicates.

Many transcription factor complexes are not stable in vitro. This step helps stablilize transcription factors and dsDNA complexes when Optical Density readings are below optimal.

(* Not supplied in all kits. This section therefore only applies to transcription factors that require stabilization. See technical manual of specific manual for more details.)

TMB (3, 3’, 5, 5’-Tetramethylbenzidine), the reagent in Ready-to-Use Substrate is provided as a ready-to-use solution. Warm to room temperature before use. Stop Solution is also provided as a ready-to-use solution.