Sigma Aldrich, Neuraminidase from Vibrio cholerae, 1 UNIT

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Type II, buffered aqueous solution, 8-24 units/mg protein (Lowry, using NAN-lactose)

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Garantie satisfait ou remboursé de 30 jours
Expédition : 2-3 jours ouvrables

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    Specifications:
    Application Protein Biology, cell Signalling
    Storage Temperature 2-8°C
    Product Type Proteins & Peptides Forms Liquid
    Product Brand Sigma-Aldrich
    Product Grade Molecular Biology

    Sialic Acid–Cleaving Enzyme for Glycoconjugate and Cell-Surface Studies

    This Type II neuraminidase from Vibrio cholerae is supplied as a buffered aqueous solution with a specific activity of 8–24 units/mg protein, determined using the Lowry method with NAN-lactose as substrate. Neuraminidases (sialidases) hydrolyze terminal sialic acid (N-acetylneuraminic acid) residues from glycoconjugates and are widely used in glycobiology, virology, and cell-surface receptor studies.

    In V. cholerae, this enzyme contains lectin-like domains flanking its catalytic center, enhancing substrate recognition and binding to complex sialylated molecules. This preparation contains protease and NAN-aldolase activity, and is preservative-free for sensitive biochemical applications.

    Product Specifications

    PropertyValue
    Product NameNeuraminidase from Vibrio cholerae (Type II)
    CAS Number9001-67-6
    EC Number3.2.1.18 / 232-624-6
    MDL NumberMFCD00131711
    Source OrganismVibrio cholerae
    FormBuffered aqueous solution
    TypeType II
    Specific Activity8–24 units/mg protein (Lowry, NAN-lactose)
    Physical FormIn 50 mM sodium acetate (pH 5.5), 0.15 M NaCl, 4 mM CaCl₂; 0.2 µm filtered
    Storage Temperature2–8 °C
    PreservativesNone
    Foreign Enzyme ActivitiesProtease and NAN-aldolase, present
    Pack Size1 unit (SKU: N6514-1UN)

    Unit Definition

    One unit will release 1.0 µmol of N-acetylneuraminic acid per minute at pH 5.0 and 37 °C using NAN-lactose or bovine submaxillary mucin as substrate. 

    Applications

    • Hydrolysis of terminal sialic acids in glycoconjugates
    • Probe for glycan structure and distribution on cell surfaces
    • Substrate specificity and lectin domain binding studies
    • Modification of tumor or immune cell surfaces for functional analysis
    • Used in virus research, including mechanisms of influenza and pathogen dissemination
    • Preparative glycan trimming for LC-MS or immunological analysis

    Supporting Literature

    1. Lectin domains assist substrate recognition: [Calorimetry Studies]
    2. Five-step purification of Vibrio neuraminidase: (J. Biochem., [1999])
    3. Leukemia cell surface modification study: (Tumor Immunol., [1988])


    Sigma-Aldrich Neuraminidase from Vibrio cholerae, Type II is a versatile sialidase suitable for glycoprotein research, cell-surface mapping, and glycoconjugate modification. With moderate specific activity and broad substrate recognition via lectin-like domains, this enzyme is ideal for functional studies in glycobiology, virology, and immunology. It provides a reliable tool for researchers investigating sialylation-dependent cell signaling, virus-host interactions, or glycoprotein structure-function relationships.

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