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| Product Name | Neuraminidase, Clostridium perfringens |
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| Description | Chromatographically purified. Neuraminidase (sialidase) splits off N-acetyl neuraminic acid (sialic acid) from a variety of glycoproteins and are important tools for the study of glycoproteins in protein chemistry and cell biology (Hatton et al. 1973). Chromatographic purification has been developed in this laboratory based on work of Cassidy et al. (1965). Wooley and Gommi (1966) describe the use of this neuraminidase in a method for measuring serotonin receptors. It is also employed to determine bound N-acetylneuraminic acid in tissues. Considerable interest has been shown in using neuraminidase inhibitors as possible anti-viral and anti-bacterial agents. Protein Content (%): ≥30% Units/Protein (u/mg): ≥10u/mg Protein A280atmg/ml: ~0.4 Assay Method: The assay is based on the measurement of sialic acid (NANA) released from bovine submaxillary mucin. One unit causes the release of one micromole of sialic acid per minute at 37°C and pH 5.0, from bovine submaxillary mucin under the speci |
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| Size | 5U, 10U |
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| Concentration | n/a |
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| Applications | n/a |
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| Other Names | EC=3.2.1.18; Clostridium perfringens |
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| Gene, Accession, CAS # | n/a |
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| Catalog # | N2100 |
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| Order / More Info | Neuraminidase, Clostridium perfringens from UNITED STATES BIOLOGICAL |
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| Product Specific References | n/a |
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