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BioReagent,For protein interaction BioReagent for sensitive chromatographic and analytical workflows requiring minimal baseline interference.
Store at 2-8°C,Room temperature,Store at -20°C,Do not freeze Ships Wet ice,Do not freeze Check lot-specific COA for exact specifications.
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Cited in 0 peer-reviewed publications across chromatography, organic synthesis, and cross-coupling reactions.
The GST Pull-Down assay is based on the reversible, specific interaction between glutathione-S-transferase (GST) and glutathione (GSH). It is used to isolate and purify unknown prey proteins using a GST-tagged bait protein. The basic principle is as follows: GSH is immobilized onto Agarose beads, forming GSH-Agarose beads. The bait protein is expressed as a fusion protein with GST, and the resulting GST−bait fusion protein can bind to the GSH-Agarose beads. If prey proteins that interact with the bait protein are present in the system, an "Agarose beads−GSH−GST-bait protein-prey protein" complex will form. This allows for the isolation and subsequent detection of the prey proteins that interact with the bait protein.
This product is manufactured by covalently coupling high−quality reduced glutathione (GSH) to Agarose beads. It features high binding capacity, rapid and convenient operation, and strong specificity. It can specifically bind to proteins containing a GST tag from sources such as cell or microbial lysates. The product offers the advantages of easy operation, high binding capability, and broad applicability.
Precautions
1. This product is intended for scientific research use by professionals only.
2. After adding GSH to the elution buffer (GSH required), the GSH contained is prone to oxidation. It is recommended to prepare the buffer fresh immediately before use .
3. Unless otherwise specified, all steps are recommended to be performed at 4°C to minimize potential protein degradation. If cell lysis is insufficient, sonication may be used after adding the lysis buffer.
4. GST-tag Purification Resin should be stored in the storage solution to prevent drying. Before use, mix thoroughly by gently inverting the tube several times to ensure uniform suspension of the beads. Avoid vigorous vortex or shaking to prevent antibody denaturation.
5. Agarose Resin that have been boiled lose their binding capacity and should not be reused.
6. Reagent volumes can be adjusted according to experimental needs. It is recommended to perform preliminary experiments to validate immunoprecipitation conditions or optimize lysis parameters.
7. Please follow safety guidelines and adhere to laboratory reagent handling protocols.
8. The lysis buffer included in this kit already contains protease inhibitors. If specific needs arise, other appropriate inhibitor cocktails can be used.
9. After harvesting, protein samples should be purified as soon as possible and kept at 4 °C or on ice at all times to minimize protein degradation and denaturation
10. It is recommended to include positive and negative control groups during immunoprecipitation or purification procedures.
G1511148 | Components | 5T | 25T | Storage Temperature | Quantity Per Test |
G1511148A | GST-tag Purification Resin | 0.2 mL | 1 mL | 2-8°C | 40 μL |
G1511148B | 1xLysis Buffer | 5 mL | 25 mL | 2-8°C | 150 μL per 250 μg sample |
G1511148C | Glutathione (Reduced, GSH) | 0.2 g | 1 g | -20°C | On request |
G1511148D | 10×BS | 10 mL | 50 mL | RT | 0.5 mL |
G1511148E | Protease Inhibitor Cocktail(100x) | 0.05 mL | 0.25 mL | -20°C | On request |
Procedure (Unless otherwise specified, all procedures should be performed at 4°C)
1.Reagent Preparation
Additional Required Materials:
(1) Reagents to be prepared by the user:
a) Primary Antibody: GST tag antibody.
b) Secondary Antibodies: Goat Anti-Mouse IgG H&L (HRP), Goat Anti-Rabbit IgG H&L (HRP).
c) Other Reagents: TBST, running buffer, transfer buffer, reducing SDS‑PAGE gel, as well as the bait protein and target protein used for protein‑protein interaction assays .
(2) Required Equipment:
Electrophoresis Apparatus, Transfer Apparatus, Imaging System
The above reagents, if required, can be ordered from Aladdin: GST Tag Mouse mAb (Ab155828), Recombinant GST tag Antibody (Ab106638), Goat Anti-Rabbit IgG H&L (HRP) (Ab176443), Goat Anti-Mouse IgG H&L (HRP)(Ab179001).
2. Solution Preparation
You may use the buffers provided in the kit, or prepare different buffer systems according to actual needs. It is recommended to filter all buffers through a 0.22 μm or 0.45 μm membrane filter before use. Buffers should be stored at 4°C. If any reagent appears cloudy, discard it immediately.
(1) Prepare an appropriate amount of inhibitor-containing lysis buffer based on the proportion of using 100-200 μL of inhibitor-containing lysis buffer for lysis and 300−600 μL of inhibitor-containing lysis buffer for washing per 0.5-1 million cells. Mix Lysis Buffer and Protease Inhibitor Cocktail (100×) at a ratio of 100:1. For example, add 10 μL of Protease Inhibitor Cocktail (100×) to 1 ml of lysis Buffer to obtain 1 ml of inhibitor-containing lysis buffer (Lysis Buffer with Protease Inhibitor Cocktail). The prepared inhibitor-containing lysis buffer should be placed on ice or at 4°C .
Note: The inhibitor-containing lysis buffer should be prepared fresh before use and should not be frozen and stored for later applications.
(2) This kit provides glutathione (GSH) powder. Weigh out 3.1 mg of the glutathione (GSH)powder using an analytical balance and add it to 1 mL of 1×PBS to prepare a glutathione elution buffer with a final concentration of 10 mM (prepare fresh before use). Then adjust the pH to neutral using NaOH.
(3) Preparation of 10×PBS: Dilute the 10×PBS with deionized water at a 9:1 ratio. For example, add 9 mL of deionized water to 1 mL of 10×PBS, and mix well to obtain the 1×PBS.
(4) GST-tag Purification Resin Washing: Gently resuspend the GST-tag Purification Resin to form a homogeneous gel suspension. Using 40 μL of well-mixed gel suspension per sample (all subsequent affinity precipitation steps use 40 μL gel suspension per sample as an example), transfer an appropriate amount of GST-tag protein purification agarose gel to a clean centrifuge tube. Add 0.5 mL of 1×PBS, centrifuge at 1250×g for 30 seconds at 4°C, discard the supernatant, and repeat this step twice.
Note: It is more convenient to aspirate the gel suspension using a wide-bore tip (e.g., by cutting off the end of a pipette tip with scissors).
3. Preparation of Bait Protein Samples (Note: Perform all sample lysis steps at 4°C or on ice)
(1)For GST-tagged fusion protein expressed in Escherichia coli:
Grow and transform E. coli according to standard protocols. Transfer 5 mL of IPTG-induced E. coli culture to a sterile centrifuge tube. Centrifuge at 5000×g for 5 minutes and discard the culture supernatant. Resuspend the pellet in 1 mL of PBS buffer per 5 mL of original culture volume, and mix by pipetting or vortex. Transfer 1 mL of cell suspension to a 1.5 mL microcentrifuge tube. Centrifuge at 5000×g for 5 minutes and discard the supernatant. Resuspend the pellet in 200 μL of ice-cold PBS buffer per 5 mL of original culture volume, and mix by pipetting or vortex. Protease inhibitors may be added as desired; for optimal results, use a protease inhibitor cocktail during cell lysate preparation. Add 200 μL of pull-down lysis buffer per 5 mL of original culture volume, and immediately invert the tube until thoroughly mixed. Incubate on ice for approximately 30 minutes, inverting the tube periodically. Centrifuge at 12000×g for 5 minutes to clarify the crude E. coli lysate. Transfer the supernatant to a new microcentrifuge tube, store on ice, and label as “bait lysate”.
(2) For secreted GST-tagged fusion protein:
Collect the culture supernatant and determine the bait protein concentration. If the bait protein concentration is high, dilute it to a final concentration of 500 μg/mL with 1×PBS for subsequent experiments.
(3) For pre-purified GST-tagged fusion protein:
Determine the bait protein concentration. If the bait protein concentration is high, dilute it to a final concentration of 500 μg/mL with 1×PBS for subsequent experiments.
Note: If the bait protein contains GSH, GSH must first be removed by dialysis or ultrafiltration before proceeding to subsequent steps.
4. Detection of Protein-Protein Interaction
(1) Immobilization of Bait Protein
1) Add the bait protein obtained in Step 3 to the pre-washed gel, mix gently, and incubate on a shaker at 4 °C for 3 h. Reserve a portion of the bait protein sample as an input control for later detection.
2) Separation by centrifugation. After incubation, centrifuge at 1250×g for 30 seconds at 4 °C, transfer the supernatant to a new centrifuge tube, and store for analysis.
3) Transfer the complex in the centrifuge tube to a spin column, centrifuge at 1250×g for 30 seconds at 4 °C, transfer the flow-through to a new centrifuge tube, and label as “bait flow-through” for later detection.
4) Add 500 μL of 1×PBS to the spin column, invert gently several times to wash the gel, centrifuge at 1250×g for 30 seconds at 4°C, and discard the eluate. Repeat 4 times to obtain the bait protein-gel complex.
(2) Capture of Target Protein.
1) Add 800 μL of the prepared prey protein sample to the bait protein-gel complex. Incubate with gentle shaking on a shaker at 4°C for at least 3 hours or overnight. Reserve a portion of the prey protein sample as a prey input for later detection.
Note: Longer incubation times may be required to ensure sufficient binding between bait and prey proteins, and can be adjusted according to experimental conditions.
2) After incubation, centrifuge at 1250×g for 30 seconds at 4 °C, transfer the flow-through to a new centrifuge tube, and label as “prey flow-through” for later detection.
3) Add 500 μL of 1×PBS to the spin column, invert gently several times to wash the gel, centrifuge at 1250×g for 30 seconds at 4 °C, and discard the eluate. Repeat 4 times to obtain the bait–prey protein–gel complex.
5. Elution of Bait–Prey Protein Complex: Elution can be performed using one of the following two methods, depending on the characteristics of the tagged protein and requirements of subsequent experiments.
(1) Non−Denaturing Elution.
Pipette 100 μL of the prepared GST elution buffer into the washed resin, mix the resin and elution buffer thoroughly, then centrifuge and collect the eluate. If elution is inefficient, increase the glutathione concentration or perform multiple elution.
(2) Elution with SDS−PAGE Loading Buffer.
For every 40 μL of original beads volume, add 50 μL of 1xPBS to resuspend the beads, followed by 50 μL of 2×SDS Loading Buffer. Mix gently by flicking the tube, then heat at 95-100°C for 5-10 minutes. Centrifuge at 1250×g for 30 seconds. Collect the supernatant for SDS-PAGE electrophoresis or Western Blot analysis.
Note: The recommended loading volume for WB is 20 μL or less. The remaining sample can be stored at -20°C.
G1511148 | Components | 5T | 25T | Storage Temperature | Quantity Per Test |
G1511148A | GST-tag Purification Resin | 0.2 mL | 1 mL | 2-8°C | 40 μL |
G1511148B | 1×Lysis Buff | 5 mL | 25 mL | 2-8°C | 150 μL per 250 μg sample |
G1511148C | Glutathione (Reduced, GSH) | 0.2 g | 1 g | -20°C | On request |
G1511148D | 10×PBS | 10 mL | 50 mL | RT | 0.5 mL |
G1511148E | Protease Inhibitor Cocktail(100x) | 0.05 mL | 0.25 mL | -20°C | On request |
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| Lot Number | Certificate Type | Date | Item |
|---|---|---|---|
| Certificate of Analysis | May 15, 2026 | G1511148 | |
| Certificate of Analysis | May 15, 2026 | G1511148 | |
| Certificate of Analysis | May 15, 2026 | G1511148 | |
| Certificate of Analysis | May 15, 2026 | G1511148 | |
| Certificate of Analysis | May 15, 2026 | G1511148 | |
| Certificate of Analysis | May 15, 2026 | G1511148 | |
| Certificate of Analysis | May 15, 2026 | G1511148 | |
| Certificate of Analysis | May 15, 2026 | G1511148 | |
| Certificate of Analysis | May 15, 2026 | G1511148 | |
| Certificate of Analysis | May 15, 2026 | G1511148 |
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