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PURECUBE NI-NTA AGAROSE NI-NTA
Home Products Cube Biotech HIS NI-NTA
PureCube Ni-NTA Agarose
Introduction
Advantages
Details
Parameter
Characteristics
Applications
Introduction
PureCube Ni-NTA Agarose

The term Ni-NTA (Nickel NTA) refers to a nickel2+ ion that has been coupled to Nitrilotriacetic acid (NTA). Ni-NTA can then be coupled to agarose resin or magnetic beads for IMAC (Immobilized Metal Chelate Affinity Chromatography). This is a purification method to obtain functional His-tagged protein. The size of the used agarose resin beads or magnetic beads influences the flow rates and the protein yield. Our PureCube Ni-NTA agarose resins are small beads with a diameter of 40 µm. They are used for the purification of active His tagged proteins from cells. Our year long experience in manufacturing agarose resin lead to the high yield of 80 mg protein per ml resin, which is leading in the market compared to other Ni-NTA suppliers. PureCube Ni-NTA resins are suited for batch spin columns and FPLC. Their small diameter provides them with a great mechanical stability. For higher flow rates we recommend our Ni-NTA agarose beads with 100 µm diameter and for extreme cases our XL sized Ni-NTA beads.

Advantages

Our year long experience in manufacturing agarose resin lead to the high yield of 80 mg protein per ml resin, which is leading in the market compared to other Ni-NTA suppliers.

Details

1. Protein Binding Capacity

The protein binding capacity is up to 70 mg/mL, as determined by purification of 6xHis-tagged GFP protein from E.coli cleared lysates, and quantified via spectrophotometry.


2.  Compatibility

PureCube Ni-NTA Agarose is very stable and can resist the following conditions in most situations: pH 2-14, 100% methanol, 100% ethanol, 8 M urea, 6 M guanidinium hydrochloride, 30% (v/v) acetonitrile.


3. High yield and purity

Our unique production process yields a Ni-NTA Agarose that exhibits a protein binding capacity >20% higher than that of two leading competitor products. Figure 1 shows the SDS-PAGE of GFP expressed in E. coli and purified in gravity colums with PureCube Ni-NTA Agarose and the Ni-NTA resin from Competitor G and Competitor Q. The protein yield in 4 elutions (E1-E4, Cube) was 80 mg/mL, compared to 65 and 48 mg/mL obtained with the alternative resins (E1-E4, Competitor G, Competitor Q). Similar results (10-18% higher binding capacity; data not shown here) were obtained comparing the purification of JNK1 (Kinase, 48 kDa) on PureCube Ni-NTA and the Ni-NTA of leading providers.

 

Fig. 1: Over 20% more yield obtained with PureCube Ni-NTA Agarose. SDS-PAGE of GFP expressed in E. coli and purified in gravity columns with PureCube Ni-NTA Agarose and Ni-NTA resin from Competitor Q. 80 mg/mL protein yield was obtained with PureCube Ni-NTA Agarose (E1–E4, Cube) compared to 65 and 48 mg/mL, respectively, with the widely used alternative resins G and Q (E1–E4, Competitor G / Competitor Q).


4.Superior DTT and EDTA stability

PureCube Ni-NTA Agarose is very robust in the presence of DTT and EDTA. In a stability test, PureCube Ni-NTA Agarose was exposed to increasing concentrations of DTT or EDTA for 1 h. Thereafter, the resins were used to purify E. coli-expressed GFP-His in gravity columns. The binding capacity of the resin decreased in the presence of both DTT and EDTA but the decay rate was shallow. In presence of DTT, PureCube Ni-NTA Agarose lost on average 8% binding capacity with each increase in DTT concentration, resulting in an overall decay of 22% at 10 mM. Even at 1.5 mM EDTA, the resin still exihibits 54% of its maximum binding capacity (Fig. 2).


Fig. 2: NTA is robust in the presence of reducing and chelating agents. GFP-His was purified on gravity columns containing PureCube Ni-NTA Agarose after exposing the resin for 1 h to 3 concentrations of DTT or EDTA. NTA exhibits a shallow decay rate in binding capacity.


5.Robust against oxidation and regenerable

PureCube Ni-NTA Agarose retains its color and function after exposure to as much as 10 mM DTT. Figure 3 shows a photo series of the resin after a 1 h exposure to 5 mM DTT. Unlike other resins, PureCube Ni-NTA Agarose did not turn brown (A). The resin was still able to bind GFP (B), with a measured binding capacity of 65 mg/mL (see Fig. 2). The resin could then be regenerated by stripping the NTA, turning the resin white (C), and reloading it with nickel ions (D). The protocol for regenerating PureCube Ni-NTA Agarose can be downloaded.

 

Fig. 3: PureCube Ni-NTA Agarose is robust against oxidation and regenerable. PureCube Ni-NTA Agarose was exposed to 5mM DTT for 1 h (A). After demonstrating that it could still bind GFP (B), the resin was washed, stripped (C), and reloaded with Ni2+ (D) following standard Cube protocol (see Cube Protocols & Datasheets).

Parameter

Type

Agarose

Ligand

NTA

Coupled Ion

Ni2+

Usage

Specific binding and purification of 6x His tagged proteins

Specifity

Affinity to His tagged proteins

Binding capacity

>80 mg/mL

Bead Ligand

Ni-NTA

Bead size

40 μm(Agarose)

Chelator stability

Stable in buffer containing 10 mM DTT and 1 mM EDTA

Filling quantity

Delivered as a 50 % suspension

Required equipment

 

-Lysis Buffer

-Wash Buffer

-Elution Buffer

-Ice bath

-Refrigerated centrifuge for 50 mL tube (min 10,000 x g)

-50 mL centrifuge tube

-Micropipettor and Micropipetting tips

-Disposable gravity flow columns with capped bottom outlet, 2 ml

-pH meter

- End-over-end shaker

-SDS-PAGE buffers, reagents and equipment Optional: Western Blot reagents and equipment

Characteristics

Order number

Products

Bead size

Binding capacity

Shipment Temperature

Storage temperature

Usage

Price(yuan)

31103

PureCube Ni-NTA Agarose(10ml)

40

80mg/mL

Ambient temperature

4° C

Use for specific binding and purification of 6x His tagged proteins;

Stable in buffer containing 10 mM DTT and 1 mM EDTA;

pH Stability: 2-14;

Max. Flow Rate: 6 mL/min

999

31105

PureCube Ni-NTA Agarose(50ml)

40

80mg/mL

Ambient temperature

4° C

3999

31110

PureCube Ni-NTA Agarose(250ml)

40

80mg/mL

Ambient temperature

4° C

15888


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Applications

Haeussler, Kristina

Journal of molecular biology 430.21 (2018): 4049-4067

Wang, Xiaoliang

ChemBioChem 19.10 (2018): 1044-1048

Volkov, Oleksandr

Science 358.6366 (2017): eaan8862

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