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脑脊液蛋白质测定:一种速率双缩脲法的评估

Assay of cerebrospinal fluid protein: a rate biuret method evaluated.

作者信息

Finley P R, Williams R J

出版信息

Clin Chem. 1983 Jan;29(1):126-9.

PMID:6848247
Abstract

We evaluated a rate colorimetric method (Beckman) for measuring total protein in cerebrospinal fluid. The automated instrument we used was Beckman's ASTRA TM. A 100-microL sample of spinal fluid is introduced into the biuret reagent in the reaction cell and the increase in absorbance at 545 nm is monitored for 20.5 s. Solid-state circuits determine the rate of alkaline biuret-protein chelate formation, which is directly proportional to the total protein concentration in the sample. The linear range of measurement is 120 to 7500 mg/L. Day-to-day precision (CV) over the range of 150 to 1200 mg/L ranged from 15.2 to 2.3%. The method was unaffected by radical alteration of the albumin/globulin ratio, but there is a positive interference in the presence of hemoglobin, a suppression in the presence of bilirubin, and no effect by xanthochromia. The method is precise, accurate, rapid, and convenient. The method was compared with the trichloroacetic acid method as performed on the Du Pont aca III, giving a correlation coefficient (r2) of 0.9693. The method is precise, accurate, rapid, and convenient.

摘要

我们评估了一种速率比色法(贝克曼法)用于测量脑脊液中的总蛋白。我们使用的自动化仪器是贝克曼的ASTRA TM。将100微升脑脊液样本引入反应池中与双缩脲试剂混合,监测545纳米处吸光度在20.5秒内的增加情况。固态电路测定碱性双缩脲-蛋白质螯合物形成的速率,该速率与样本中的总蛋白浓度成正比。测量的线性范围是120至7500毫克/升。在150至1200毫克/升范围内的日间精密度(CV)为15.2%至2.3%。该方法不受白蛋白/球蛋白比例剧烈变化的影响,但在存在血红蛋白时有正干扰,在存在胆红素时有抑制作用,而黄变则无影响。该方法精确、准确、快速且方便。将该方法与在杜邦aca III上进行的三氯乙酸法进行比较,相关系数(r2)为0.9693。该方法精确、准确、快速且方便。

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