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作 者:文翔昊[1] 李冲[1] 郭露[1] 鲁启明[1] 孙林军[2] 郭玉[2]
机构地区:[1]南华大学附属南华医院,湖南衡阳421002 [2]南华大学药物药理研究所,湖南衡阳421001
出 处:《广东化工》2014年第22期146-147,157,共3页Guangdong Chemical Industry
基 金:湖南省中医药局重点课题项目;编号:201211
摘 要:目的:建立溴化乙锭(EB)与脱氧核糖核酸(DNA)的共振光散射光谱法测定生物样本DNA的含量。方法:在含一定量EB的PBS磷酸缓冲溶液(p H 3.5)中,依次加入不同浓度的DNA,检测该体系的共振光散射强度。结果:在波长为363.0 nm处,存在一共振光散射增强峰,其增强强度(IRLS=I-I0)与DNA浓度呈明显的线性关系。线性方程为ΔIRLS=2.8711CDNA+5.435,R=0.9955,方法的线性范围为0.025~50.8μg/m L,检出限为0.5 ng/m L。结论:本实验建立的EB-DNA共振光散射法是一种灵敏高、适用于生物样本中DNA含量的简便方法。Objective: To establish the resonance light scattering spectroscopy method of ethidium bromide(EB) and deoxyribonucleic acid(DNA) for measureing DNA content in biological samples. Methods: Using resonance light scattering(RLS) method, the RLS signals of the systems containing amount EB and different concentrations of DNA were detected in p H 3.5 PBS buffer solution. Results: At a wavelength of 363.0 nm, there is an enhanced resonance light scattering peak which was remarkably increases after the addition of DNA. The results showed a linear relationship between the enhanced RLS intensity of the EB-DNA system and DNA concentration. The linear regression equation is represented as follows: ΔIRLS=2.8711CDNA+5.435,with regression coefficient R=0.9955. The detection limit was 0.5 ng m L-1. Conclusion: The method established of EB-DNA resonance light scattering is a highly sensitive, simple and suitable for determining DNA content in biological samples.
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