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A direct, competitive enzyme-linked immunosorbent assay (ELISA) as a quantitative technique for small molecules

机译:直接竞争的酶联免疫吸附测定(ELISA)作为小分子的定量技术

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摘要

ELISA (enzyme-linked immunosorbent assay) is a widely used technique with applications in disease diagnosis, detection of contaminated foods, and screening for drugs of abuse or environmental contaminants. However, published protocols with a focus on quantitative detection of small molecules designed for teaching laboratories are limited. A competitive, direct ELISA used to detect and quantify levels of digoxin, a cardiac glycoside, is described. Unique features of this lab include collecting data in quadruplicate followed by statistical analysis of replicates using a Q-test. Use of a microplate reader for measuring absorbances makes data collection extremely quick. Students plot their average absorbance versus log concentration digoxin and fit data to a third- or fourth-order polynomial. They also examine the maximum and minimum absorbance for the assay, determine the region of linearity, and then fit the linear region to a straight-line equation that can be used to determine the concentration of an unknown. The experiment can be completed in a 3-h period and is suitable for upper-level biochemistry, chemistry, and biology students. Although students find understanding a competitive ELISA more challenging than some other experiments, they enjoy learning about this commonly used laboratory technique.
机译:ELISA(酶联免疫吸附测定)是一种广泛使用的技术,可用于疾病诊断,污染食品的检测以及滥用药物或环境污染物的筛选。但是,为教学实验室设计的,侧重于小分子定量检测的已公开协议是有限的。描述了用于检测和定量地高辛(强心苷)水平的竞争性直接ELISA。该实验室的独特功能包括一式四份收集数据,然后使用Q检验对重复数据进行统计分析。使用微孔板读取器测量吸光度可以非常快速地收集数据。学生绘制平均吸光度与对数浓度地高辛的关系图,并将数据拟合为三阶或四阶多项式。他们还检查了测定的最大和最小吸光度,确定了线性区域,然后将线性区域拟合到可用于确定未知浓度的直线方程。实验可以在3小时内完成,适合高级生物化学,化学和生物学专业的学生。尽管学生发现了解竞争性ELISA比其他一些实验更具挑战性,但他们仍喜欢这种常用的实验室技术。

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