Isolation of the Cytotoxic Glycoprotein by Lectin Affinity Chromatography (CAT#: STEM-ACM-0021-CJ)

Introduction

Glycosylation as a common post-translational modification of proteins is an important function-related structural characteristic in cytotoxic substances. Snake, fish, mollusc and scorpion venoms are known to contain glycoproteins as active compounds. Carbohydrate side chains of glycoproteins in snake venoms acting as anticoagulant factors have been characterized due to their affinity to lectins of different specificity.

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Principle Applications Procedure Materials Notes Related Products

Principle

In general affinity chromatography is composed of a stationary phase (solid phase) and a mobile phase. The mobile phase is the cell lysate or any mixture that contains biomolecules. A ligand that binds the target molecule is attached covalently to the solid phase. The interaction between the solid and the mobile phase are exploited by affinity chromatography to get your desired substance in a pure form. The target molecule binds to the ligand, whereas most of the other molecules flow through. The target biomolecule is eluted by changing conditions (pH or salt concentrations) or by competition with a free ligand.The most important property which the solid phase should have is ligand immobilization. Various materials like acrylates or silica gels are appropriate. To prevent steric interference of the target molecule to the ligand, an inhibitor is attached to the solid phase. This inhibitor is known as the spacer.

Applications

Cell Biology; Biochemical

Procedure

1. Preparation of Column: The column is loaded with solid support such as sepharose, agarose, cellulose etc.. Ligand is selected according to the desired isolate. Spacer arm is attached between the ligand and solid support.
2. Loading of Sample: Solution containing a mixture of substances is poured into the elution column and allowed to run at a controlled rate.
3. Elution of Ligand-Molecule Complex: Target substance is recovered by changing conditions to favor elution of the bound molecules.

Materials

• Sample: Plants; Natural Food; Protein; Drug; Pollutants; Blood; Saliva; Serum; Plasma; Antibodies; Viruses & More
• Equipment: Agarose; Silica gel; Aluminium oxide; Acrylate; Organic polymers; Wash Buffer
• (Optional): Ligand; Spacer arm; Column

Notes

1. Due to the ability of all lectins to identify and bind certain types of carbohydrate residues, this approach can be used to separate them.
2. The most common lectins employed in affinity columns are concanavalin A, soybean lectin, and wheat germ agglutinin.
3. Bioaffinity chromatography types can also utilise enzymes, inhibitors, cofactors, nucleic acids, hormones, and cell chromatography as ligands.

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