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HomeZymo Research Products P2001 His-Spin Protein Miniprep
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P2001 His-Spin Protein Miniprep

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SKU: P2001 Category: Zymo Research Products
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Description

Highlights

  • Fast: Purify His-tagged proteins from cell lysates in less than 5 minutes.
  • Simple: Prepare pure protein for small-scale studies using a spin-column.
  • Convenient: No special instrumentation needed other than a benchtop microcentrifuge.

Description

The P2001 His-Spin Protein Miniprep provides a fast spin-column based purification technology for His-tagged proteins. Up to 1 mg of His-tagged protein can be purified in 5 minutes and eluted in as little as 100 ?l of His-Elution Buffer. The purified protein is ultra-pure and can be used directly for enzymatic assays, protein biochemical analyses, SDS-PAGE and other sensitive applications. The straightforward spin, wash, and elute protocol dramatically simplifies protein purification and allows the end user to get results in minutes, not hours.

Technical Specifications

Affinity Matrix

Nickel charged agarose

Binding Capacity

1 mg

Elution Method

Imidazole gradient

Elution Volume

100 – 200 µl (150 µl is optimal)

Principle of Technology

Based on a nickel-charged His-Affinity Gel (IMAC).

Processing Time

5 minutes

Product Storage

Please store the His-Affinity Gel, His-Binding Buffer, His-Wash Buffer, and His-Elution Buffer at 4?C. The other components can be stored at room temperature.

Protein Purity

Electrophoretically pure. Purified high-quality protein is suitable for enzyme kinetics, protein biochemical analyses, SDS-PAGE, and other applications.

Required Equipment

Microcentrifuge

Sample Type

Cell lysates or other complex protein mixtures containing His-tagged proteins.

Product FAQ

Q1: Is the product suitable for eukaryotic expression system (HEK cells)?

Yes, the His-Spin Protein Miniprep Kit can also be used with eukaryotic expression systems. For references: Marcos J. Caballero-L?opez, Manuel Nieto-D??az, M?onica Yunta, David Reigada, Teresa Mu?noz-Galdeano, ?Angela del ?Aguila, Rosa Navarro-Ru??z, Wolfang Pita-Thomas, Dan Lindholm, Rodrigo M. Maza – XIAP Interacts with and Regulates the Activity of FAF1 ? 2017, BBA – Molecular Cell Research. doi:10.1016/j.bbamcr.2017.04.006

Q2: Can less than 100 ?l of His-Elution Buffer be used for the elution step?

Smaller elution volumes are possible and may yield more concentrated protein, but the elution efficiency may be compromised.

Q3: What might reduce protein yields?

– The His-tag may be rendered inaccessible due to protein folding. The protein can be purified at denaturing conditions. – The recombinant protein can become insoluble as a result of overexpression. The protein can be purified at denaturing conditions. – Starting material is too dilute. If the starting material contains very low levels of His-tagged protein, then it may require more than 300 ?l of sample volume to purify enough protein. Simply repeat steps 3 and 4 until the desired volume has been loaded onto the column. – The protein is bound to the His-Affinity Gel too tightly and can not be eluted with the supplied His-Elution Buffer. A custom-made elution buffer containing 500 mM imidazole or 100 mM EDTA may elute the tightly-bound protein. – Depending on the protein, lowering the imidazole concentration of the His-Wash Buffer to 25 mM (e.g., by dilution with His-Binding Buffer) may increase yields.

Q4: Which chemicals/reagents are not compatible with the kit?

EDTA, EGTA, DTT, > 15 mM ?-mercaptoethanol, and > 10 mM imidazole or histidine. If your starting material contains these compounds, dilution with the His-Binding Buffer may help. Multiple loadings on the column will be necessary to load enough material. If the sample is in a different buffer, adjust the pH and imidazole and salt concentrations and carry out a test preparation. If the protein is still not bound, the sample needs to be dialyzed before use.

Q5: How do you purify insoluble proteins?

– Optimize expression conditions. Overexpression of proteins may result in formation of insoluble inclusion bodies inside cells. If a large band of overexpressed protein is visible after SDS-PAGE electrophoresis of whole cells, but the band is absent after SDS-PAGE electrophoresis of cleared cell lysates, this indicates that the protein may not be soluble and the expressed protein may form inclusion bodies. – Use Denaturing conditions. Insoluble proteins will not be purified using the provided buffers. It is, however, possible to purify such proteins at denaturing conditions in the presence of ? 8 M urea or ? 6 M guanidine hydrochloride. The protein native structure and thus enzyme activity is lost under such conditions, but may be restored by refolding the protein after purification.

Q6: Can the kit be used to purify membrane proteins?

Membrane proteins can be purified after solubilization in a nonionic detergent. Concentrations of up to 2% of Triton? or TWEEN? can be present in the loaded sample.

Q7: Which pH should be used with the kit?

The pH value of the loaded sample should be between 7.5 and 8.0. Too high or low pH can result in decreased protein yields and/or quality.

Q8: How do you improve protein quality/purity?

– Check your buffers for signs of contamination and check the pH of the buffers. – Increase centrifugation time and speed. Ensure that the His-Affinity Gel drains completely after each spin (some older centrifuge models may require a longer centrifugation time). – If the problem persists, additional wash steps can be added to the purification protocol, or increasing the imidazole concentration of the washing buffer to 60 ? 100 mM (e.g., by dilution with the His-Elution Buffer).

Q9: Is there a recommended lysis protocol?

Is there a recommended lysis protocol? For protein purification from?E. coli?lysates: 1. Harvest & pellet 10 ml of?E. coli?culture. 2. Resuspend in 1 ml of His-Binding Buffer. 3. Lyse the cells by sonication (or other methods). 4. Spin at ? 12,000?x g?at 4?C for 5 minutes. 5. Use 150 ?l of the supernatant for the His-Spin Protein Miniprep protocol.

Q9: Is there a recommended lysis protocol?

Is there a recommended lysis protocol? For protein purification from?E. coli?lysates: 1. Harvest & pellet 10 ml of?E. coli?culture. 2. Resuspend in 1 ml of His-Binding Buffer. 3. Lyse the cells by sonication (or other methods). 4. Spin at ? 12,000?x g?at 4?C for 5 minutes. 5. Use 150 ?l of the supernatant for the His-Spin Protein Miniprep protocol.

Q10: Which chemicals/reagents are compatible with the kit?

Reducing Agents ? 15 mM ?-mercaptoethanol Non-Ionic Detergents ? 2% Nonidet? P-40 ? 2% Triton? X-100 ? 2% Tween?-20 Denaturing Reagents ? 8 M Urea Chemicals and other Reagents ? 10 mM Imidazole ? 10 mM Histidine

Citation

96?/ 100
Bioz Stars

The Robust Self-Assembling Tubular Nanostructures Formed by gp053 from P…

Viruses – Published 11 Jan 2019

The recombinant His-tagged protein purification using the metal-chelating sorbent was performed by using the His-Spin Protein Miniprep kit (Zymo Research, Irvine, CA, USA) according to the manufacturer?s recommendations.. The concentration of the recombinant protein was determined by using a method described by Lowry.

Genomic Characterization of Cyanophage vB_AphaS-CL131 Infecting Filament…

Appl Environ Microbiol – Published 13 Dec 2018

Supernatant and pellets were directly analyzed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE).. Recombinant His-tagged proteins were purified using a His-Spin Protein Miniprep kit (Zymo Research) according to the manufacturer’s recommendations.. Concentration of recombinant protein was determined with electrophoresis and by using the method described by Lowry et al.

A modified serine cycle in Escherichia coli coverts methanol and CO2 to …

Nat Commun – Published 28 Sep 2018

Cell pellet was lysed with 0.1 mm diameter glass beads at 4 ?C, and protein was purified by His-Spin Protein Mini-prep columns (Zymo Research).. Concentration of purified protein was measured using BioRad Protein Assay kit, and protein purity was verified by standard SDS-PAGE with Coomassie

See more details on Bioz

Reviews

?I?m a Zymo fan! DNA/RNA Shield is a great product. It works great on my precious samples. I trust Zymo Research products and they have great tech support!!?

– Laura T. (USDA)

?We use DNA/RNA shield and it works well with adults mosquitoes, larvae, eggs. We store it at RT for weeks and at -4?C or -20?C for months, never saw any DNA degradation.?

– Umberto P. (University of Pavia)

?I did an assay using RNA/DNA shield and it works perfect. The product have excellent reproducibility when stored at 4?C for up to a month.?

– Maha AE. (University of Florida)

?We extracted RNA from cells suspended in DNA/RNA Shield with the Direct-zol miniprep set from Zymo (using Trizol). It worked perfect for us.?

– Mariska B. (University of Amsterdam)

Kit Components

Cat # Name Size
P2003-2 His-Affinity Gel 14 ml
P2003-3 His-Binding Buffer 50 ml
P2003-4 His-Wash Buffer 50 ml
P2003-5 His-Elution Buffer 25 ml
C1001-50 Collection Tubes 50 Pack
P2003-1 Zymo-Spin P1 Columns 50 Pack

Additional Information

  • Catalog#: P2001 /P2002
  • Package Length (in Inches):7
  • Package Width (in Inches): 3 /5
  • Package Height (in Inches): 1.3 /4.5
  • Package Weight (in Pounds): 0.3 /1.05
  • Size: 10 Prep /50 Prep
  • Unit Standard: Metric
  • Volume Units: Milliliters
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