Acta Chimica Sinica ›› 2011, Vol. 69 ›› Issue (18): 2153-2158. Previous Articles     Next Articles

Full Papers

双链DNA裂解-纳米金共振散射光谱探针检测痕量 UO22+  

张轶,梁爱惠*,周莲平,覃惠敏,欧阳辉祥,王鹏飞,蒋治良*   

  1. (广西师范大学环境与资源学院 广西环境工程与保护评价重点实验室 桂林 541004)
  • 投稿日期:2010-11-04 修回日期:2011-04-10 发布日期:2011-05-03
  • 通讯作者: 蒋治良 E-mail:zljiang@mailbox.gxnu.edu.cn
  • 基金资助:

    国家自然科学基金

Double Stranded DNA Cleaved-nanogold Resonance Scattering Spectral Probe for Assay of Trace UO2 2+

ZHANG Yi, LIANG Ai-Hui, ZHOU Lian-Ping, QIN Hui-Min, 欧Yang-Hui-Xiang , WANG Peng-Fei, JIANG Zhi-Liang   

  1. (Guangxi Key Laboratory of Environmental Engineering and Protection Assessment, School of Environment and Resource Sciences, Guangxi Normal University, Guilin 541004)
  • Received:2010-11-04 Revised:2011-04-10 Published:2011-05-03

In pH 5.5 2-(N-morpholine)-ethyl sulfonic acid buffer solution and in the presence of NaCl, the substrate single stranded DNA hybridized with the DNA enzyme to form double stranded DNA (dsDNA) at 80 ℃. can cleaved the substrate strand of the dsDNA to produce short single stranded DNA that adsorbed on the surface of the gold nanoparticle to prevent its aggregation, and the uncombined gold nanoparticles aggregate to big particles that exhibited a resonance scattering (RS) peak at 610 nm. When the concentration increased, the short single stranded DNA increased, the combined gold nanoparticles increased, and the aggregated gold nanoparticles decreased, the RS intensity at 610 nm decreased. Under the selected conditions, the decreased RS intensity (ΔI610 nm) is linear to concentration in the range of 0.67~60.3 nmol/L, with a regression equation of ΔI610 nm=11.9C+6.1, a correlation coefficient of 0.9972, and a detection limit of 0.09 nmol/L . This method has been applied to determination of in wastewater, with satisfactory results.

Key words: aptamer, double stranded DNA, nanogold, resonance scattering spectral assay