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CAS RN: | Product Number: R0235
rPSL1a-LecBeads [for Siaα(2-6)Gal]
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Purity:
Synonyms:
- rPSL1a-Agarose
- Recombinant Polyporus squamosus lectin (= rPSL1a)-Agarose
Product Documents:
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Supplemental Product Information:
Product information
Product code : R0235
Product name : rPSL1a-LecBeads [for Siaα(2-6)Gal]
Preparation : Recombinant PSL1a is covalently coupled with agarose gel
Quantity : 1 ml gel/2 ml (1:1, v/v slurry) suspended in PBS, pH7.5
Protein concentration : about 10 mg/ml gel
Binding capacity : >10 mg of glycoprotein (human Transferrin) /ml gel
Preservative : 0.02% [w/v] Sodium azide
Stabilizer : None
Description
The rPSL1a is an Escherichia coli recombinant of carbohydrate-binding protein (Lectin) derived from Polyporus squamosus. This lectin preferably binds to a [Siaα(2-6)Gal] glycan epitope (It very slightly interacts with lactose.).
The LecBeads is a lectin-immobilized agarose which is capable of capturing glycoproteins via binding to its specific epitope(s), and it is prepared by a covalent coupling method between lectin and agarose.
The Lectin-catch method using LecBeads (as shown in Application tab) is available for selective separation of glycoconjugates (glycoproteins, glycolipids, and so on). This rPSL1a-LecBeads (1 ml gel) shows a binding capacity of about 10 mg or more human Transferrin [hTF] through its binding to a terminal [Siaα(2-6)Gal] glycan epitope on hTF.
Storage
Store at 2-10°C. (Avoid freezing).
Related Products
R0225 Recombinant Polyporus squamosus lectin (rPSL1a) expressed in Escherichia coli
R0230 rPSL1a-Biotin [for Siaα(2-6)Gal]
R0236 rLSL-N-LecBeads [for Galβ(1-4)GlcNAc, poly LacNAc]
R0237 rMOA-LecBeads [for Galα(1-3)Gal]
R0238 rSRL-LecBeads [for GlcNAcβ(1-2)Man, Galβ(1-3)GalNAc]
R0239 rGRFT-LecBeads [for Manα(1-2)Man]
A3331 AOL-LecBeads [for Fucα(1-6)/α(1-4)/α(1-3)/α(1-2)]
| Product Number | R0235 |
| Physical State (20 deg.C) | Liquid |
| Storage Temperature | Refrigerated (0-10°C) |
| Condition to Avoid | Heat Sensitive |
Specifications
| Appearance | White to Almost white clear liquid to cloudy liquid |
| Concentration(Lowry method) | min. 9.0 mg/mL gel |
| Binding capacity | to pass test(min. 10 mg/mL gel, Human Transferrin) |
Properties (reference)
GHS
Related Laws:
Transport Information:
| H.S.code* | 3504.00-000 |
Application
The lectin-catch procedure
< Preparation >
Buffers
Binding buffer : PBS pH7.5
Elution buffer : PBS pH7.5 containing 200 mM lactose [Product code: L0008] and 0.1% triton-X100 [Product code: P1775]
< Method of the lectin-catch > ※Centrifuge method
Equilibration
- Prepare the LecBeads in a new tube.
- Add the Binding buffer into the tube to equilibrate the gel.
- Centrifuge the tube at 800 ×g for 3 min and discard the supernatant. (If necessary, repeat equilibration with the Binding buffer >10-fold volume of the LecBeads appropriately.)
Binding
- Concentrate or dilute the glycoprotein sample to moderate concentration (e.g., 1 mg/ml) with the Binding buffer [Input fraction], and apply the prepared sample to the tube in which the LecBeads was preliminary equilibrated.
- Agitate the tube at 4°C (※Generally, a dissociation constants (Kd value) of lectins are tend to be decreased at lower temperature) for a few hours (or overnight).
- Centrifuge the tube at 800 ×g for 3 min and remove the supernatant [Through fraction].
- Wash the LecBeads by 5 (to 10)-fold of the slurry volume with the Binding buffer several times.
Elution
- Elute the glycoprotein from the LecBeads by agitation with an appropriate volume of the Elution buffer (e.g. same volume of the LecBeads).
- Agitate the reaction tube at 4°C or R.T. for a few hours (or overnight).
- Centrifuge the tube at 800 ×g for 3 min and remove the supernatant [Elution fraction].
- Check the resulting fractions ([Input fraction] [Through fraction] [Elution fraction]) by protein assay and SDS-PAGE. (In some cases, the repetitive elution step with a small volume of the Elution buffer might improve the elution effect. If necessary, repeat elution steps.)
- The competitive oligosaccharide included in the obtained elution fractions can be removed by ultrafiltration or dialysis using a sufficient amount of buffer.
References
- Glyco-catch method: A lectin affinity technique for glycoproteomics
- Separation technologies for glycomics
Articles/Brochures
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