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C-His tag Nanoselector Agarose

Details and Advantages
Applications: IP,CHIP,MS,Purification
Reactivity: His tag
Conjugate: Agarose
Advantages:

· Consistent and reproducible results

· No heavy & light antibody chains

· Extraordinary binding, even under harsh conditions

· High affinity

· Short Incubation (5-30 min)

Summary >

Description: 

C-His tag Nanoselector Agarose have been specifically designed to bind His tag-fusion proteins. His tag Nanoselector Agarose is based on small high-affinity recombinant alpaca antibody fragments covalently coupled to the surface of Agarose. His tag Nanoselector Agarose is an ideal tool to isolate or purify His tag-fusion proteins fast and efficiently.

Ligand: Anti-His tag(C-terminal) single domain antibody fragment (VHH, Nanobody)

Bead size: ~ 40 µm

Reactivity: The C-His tag-Nanoselector recognizes the His-tag sequence motif HHHHHH at the C-terminus of the fusion protein.

Binding capacity: High binding capacity, 10 µL slurry bind about 20µg of recombinant GFP-His protein.

Storage: Shipped at ambient temperature. Upon receipt store at 4°C. Stable for 1 year. Do not freeze.

Storage buffer: Formulation 50 % slurry in PBS containing 20 % Ethanol.



Background:

His-tag, or polyhistidine tag, comprises a consecutive series of six to ten histidine residues. The size of the His tag is small and it hardly affects the functionality of the fusion protein. His tag is widely used for many recombinant proteins to facilitate purification, and allows researchers to purify the protein of interest from cell lysate or mixture of many proteins easily .

His tag Nanoselector Agarose has been specifically designed to bind His tag. Due to the single-chain nature of sdAbs and their stable and covalent attachment, no leakage of light and heavy chains is observed during elution with SDS sample buffer. His tag Nanoselector Agarose thus features high affinity and superior capacity for His tag fusion proteins while showing negligible non-specific background. His tag Nanoselector Agarose is compatible not only with physiological buffers but also with high stringency buffers which provides great freedom to adjust the binding and washing conditions to the experimental needs.


Performance >

Immunoprecipitation (IP)/Co-IP
Mass spectrometry (MS)
Enzyme activity measurements

Experimental scheme >

Immunoprecipitation protocol

 

Mammalian cell lysis

Note: Harvesting of cells and cell lysis should be performed with ice-cold buffers. We strongly recommend to add protease inhibitors to the Lysis buffer to prevent degradation of your target protein and its binding partners.

For one immunoprecipitation reaction, we recommend using ~106- 107 cells.

1. Choice of lysis buffer:

* For cytoplasmic proteins, resuspend the cell pellet in 200 µL ice-cold Lysis buffer by pipetting up and down. Supplement Lysis buffer with protease inhibitor cocktail and 1 mM PMSF (not included).

* For nuclear/chromatin proteins, resuspend cell pellet in 200 µL ice-cold RIPA buffer supplemented with DNaseI (f.c. 75-150 Kunitz U/mL), MgCl2 (f.c. 2.5 mM), protease inhibitor cocktail and PMSF(f.c. 1 mM)(not included)

2. Place the tube on ice for 30 min and extensively pipette the suspension every 10 min.

3. Centrifuge cell lysate at 17,000x g for 10 min at +4°C. Transfer cleared lysate (supernatant) to a pre cooled tube and add 300 µL Dilution buffer supplemented with 1 mM PMSF and protease inhibitor cocktail (not included). If required, save 50 µL of diluted lysate for further analysis (input fraction).

 

Bead equilibration

1. Resuspend the beads by gently pipetting up and down or by inverting the tube. Do not vortex the beads!

2. Transfer 25 µL of bead slurry into a 1.5 mL reaction tube.

3. Add 500 µL ice-cold Dilution buffer.

4. Sediment the beads by centrifugation at 2,500x g for 5 min at +4°C.

5. Discard the supernatant.

 

Protein binding

1. Add diluted lysate to the equilibrated beads.

2. Rotate end-over-end for 1 hour at +4°C.

 

Washing

1. Sediment the beads by centrifugation at 2,500x g for 5 min at +4°C.

2. If required, save 50 µL of supernatant for further analysis(flow-through/non-bound fraction).

3. Discard remaining supernatant.

4. Resuspend beads in 500 µL Wash buffer.

5. Sediment the beads by centrifugation at 2,500x g for 5 min at +4°C. Discard the remaining supernatant.

6. Repeat this step at least twice.

7. During the last washing step, transfer the beads to a new tube.

 

Optional: To increase stringency of the Wash buffer, test various salt concentrations e.g. 150 mM - 500 mM,and/or add a non-ionic detergent e.g. Triton™ X-100.

 

Elution with 2x SDS-sample buffer

1. Remove the remaining supernatant.

2. Resuspend beads in 80 µL 2x SDS-sample buffer.

3. Boil beads for 5 min at +95°C to dissociate immunocomplexes from beads.

4. Sediment the beads by centrifugation at 2,500x g for 2 min at +4°C.

5. Analyze the supernatant in SDS-PAGE.

 

Elution with Glycine-elution buffer

1. Remove the remaining supernatant.

2. Add 50–100 µL Glycine-elution buffer and constantly pipette up and down for 30 - 60 sec at +4°C.

3. Sediment the beads by centrifugation at 2,500x g for 5 min at +4°C.

4. Transfer the supernatant to a new tube.

5. Immediately neutralize the eluate fraction with Neutralization buffer.

6. Repeat this step at least once to increase elution efficiency .