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首页> 外文期刊>Clinical Chemistry: Journal of the American Association for Clinical Chemists >Rapid electrophoretic determination of neuron-specific enolase isoenzymes in serum.
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Rapid electrophoretic determination of neuron-specific enolase isoenzymes in serum.

机译:血清中神经元特异性烯醇酶同工酶的快速电泳测定。

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摘要

This assay procedure for each of the two neuron-specific enolases (alpha gamma and gamma gamma) and the non-neuronal enolase (alpha alpha) in serum involves two steps: electrophoretic separation of the three isoenzymes--alpha alpha, alpha gamma, and gamma gamma--on cellulose acetate, and bioluminescence measurement of total enolase activity. From these data, the activity concentrations (U/L) of the three isoenzymes in serum are calculated. Both measurement steps are based on the enzymatic activity of enolase and thus differ from the immunological methods currently in use, which require the availability of specific antibodies. The method is rapid (approximately 30 min for both steps) and requires only 10 microL of serum for the complete analysis. Studies of normal children and adults, and of patients suffering from neuroblastoma and small-cell lung cancer, show that it is suitable for clinical use. Furthermore, the fact that both neuron-specific isoenzymes of enolase can be systematically separated is an advantage over immunological techniques in determining isoenzyme patterns for pathological samples.
机译:该测定方法对于血清中的两个神经元特异性烯碱基(αγ和γγ)和非神经元烯醇酶(αα)中的每一个涉及两个步骤:三个同工酶的电泳分离 - ααα,αγ和γγ-乙酸纤维素,以及总烯醇酶活性的生物发光测量。从这些数据中,计算血清中三种同工酶的活性浓度(U / L)。两个测量步骤都基于烯醇酶的酶活性,因此与目前使用的免疫学方法不同,这需要特异性抗体的可用性。该方法快速(两个步骤约30分钟),只需要10微升血清进行完整分析。对正常儿童和成人的研究,以及患有神经母细胞瘤和小细胞肺癌的患者,表明它适用于临床用途。此外,可以系统地分离烯醇酶的神经元特异性同工酶的事实是在确定病理样品中的同工酶模式中的免疫技术具有免疫技术的优点。

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