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机构地区:[1]浙江建安检测研究院有限公司,杭州310021 [2]中国药科大学药学院,南京210009 [3]安庆师范学院化学化工学院,安庆246001
出 处:《应用化学》2013年第2期225-231,共7页Chinese Journal of Applied Chemistry
基 金:安徽省教育厅基金资助项目(2008jp1101);中国药科大学博士科研启动项目(211166)
摘 要:室温下一步合成了一种蓝色发光金量子点。该金量子点具有良好的水溶性和生物相容性,金量子点平均粒径为3.0 nm,在波长305 nm光激发下,发射430 nm蓝色荧光。实验发现,一定量L-半胱氨酸对金量子点430 nm处荧光发射有显著的增强作用,由此可建立一种简单、迅速、灵敏检测L-半胱氨酸的新方法。在最佳条件下,金量子点荧光强度与L-半胱氨酸在0~4.0μmol/L浓度范围内呈线性关系,线性相关系数R2=0.9976,对2.0μmol/L L-半胱氨酸的11次测定结果的相对标准偏差(RSD)为2.8%,以3倍标准偏差计算本法对L-半胱氨酸测定的检出限为5 nmol/L。Blue luminescent gold (Au) quantum dots (QDs) were facilely prepared through a one-pot synthesis at room temperature. The as prepared Au QDs were well water-soluble and biocompatable. The mean size of Au QDs is about 3.0 nm. Gold QDs colloids showed a considerable blue fluorescence emission at 430 nm under excitation of 305 nm. Experimental results demonstrated that the addition of L-cysteine could significantly enhance the characteristic emission of Au QDs at 430 nm. Therein, a simple, rapid, sensitive detection of L-cysteine in aqueous solution was established. Under optimized conditions, the characteristic fluorescence intensity of Au QDs at 430 nm is linearly proportional to the concentration of L-cysteine in the range of 0. 0 to 4. 0 × 10 -6 μmol/L and a detection limit as low as 5 nmol/L was obtained. The relative linear relationship coefficient is 0. 9976. The relative standard deviation for 11 replicate detections of 2.0μmol/L L-cysteine was 2.8%. In addition, this method also demonstrated a high selectivity to amino acids due to the strong affinity of L-cysteine to gold atoms.
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