Sialidase assay by luminescence in the low picomole-range of sialic acid. Its application to the measurement of this activity in influenza virus.

Hoppe-Seyler's Zeitschrift fur physiologische Chemie Pub Date : 1984-04-01 DOI:10.1515/bchm2.1984.365.1.415

J A Cabezas, N Pérez, M Llanillo, A Reglero, P Calvo

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引用次数: 4

Abstract

A new procedure for a sialidase assay, by bioluminescence, has been developed. The substrate, N- acetylneuraminyllactose (sialyllactose), hydrolysed by the sialidase activity, releases lactose. This lactose is hydrolysed with beta-galactosidase. The released galactose is oxidized with galactose dehydrogenase and NAD. The NADH produced in the last step is measured by a luminescence system, coupling two enzymes, NAD(P)H dehydrogenase (FMN) and luciferase. This microassay, which is specific, rapid, simple and ultra-sensitive, is a measure for amounts as little as (at least) 5 pmol of N-acetylneuraminic acid (corresponding to 0.15 ng of the released sialic acid). It uses commercialized reagents (non-radioisotopic) and avoids interferences common in other procedures. This method has been used for measuring sialidase activity directly on intact virus, avoiding inconvenient modifications produced in the extraction of the enzyme. The specific activity of sialidase of influenza virus X31 (H3N2), determined by this procedure, is 0.65 U/mg of total virus protein.

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发光法测定唾液酸低皮摩尔范围的唾液酸酶。应用于流感病毒中这种活性的测定。

一个新的程序唾液酸酶测定，生物发光，已经开发。底物N-乙酰神经胺基乳糖(唾液基乳糖)被唾液酶活性水解，释放乳糖。这种乳糖用-半乳糖苷酶水解。释放的半乳糖被半乳糖脱氢酶和NAD氧化。最后一步产生的NADH通过耦合NAD(P)H脱氢酶(FMN)和荧光素酶两种酶的发光系统来测量。该微量分析具有特异、快速、简单和超灵敏的特点，可检测少量(至少)5 pmol的n -乙酰神经氨酸(相当于0.15 ng唾液酸)。它使用商业化的试剂(非放射性同位素)，避免了其他程序中常见的干扰。该方法可直接在完整病毒上测定唾液酸酶活性，避免了提取唾液酸酶时产生的不便修饰。用该方法测定流感病毒X31 (H3N2)唾液酸酶的比活性为0.65 U/mg。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Hoppe-Seyler's Zeitschrift fur physiologische Chemie

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