氢化物发生-原子荧光光谱法测定铜精矿中的砷、锑和铋

建立了氢化物发生-原子荧光光谱法同时测定铜精矿中砷、锑、铋的方法,采用了主量元素匹配法来消除基体干扰,优化了反应体系的酸度、还原剂浓度等条件进行了优化。砷、锑、铋的浓度在1—200μg·L~(-1)范围内与荧光强度呈线性关系。方法回收率为92%—101%,相对标准偏差为2.7%—5.5%。     

平行因子-同步荧光法测定食品中维生素B1,B2和B6

文章应用同步荧光法对维生素B1、B2和B6的混合物进行了分析。由于维生素B的荧光波谱存在重叠本工作采用三维同步荧光技术结合平行因子分析法（PARAFAC）,对维生素B1,B2和B6混合物的三维荧光数据进行了测定和解析,并以高效液相色谱法（HPLC）作对照,获得了较好的结果。实验中取Ex=200～500nm和△λ=20～120nm。     

基于荧光分析的氨基甲酸酯类农药残留检测系统

通过对氨基甲酸酯类农药在紫外光照射下能够产生荧光的机理研究,设计了一种用于检测氨基甲酸酯类农药残留的荧光系统。该系统采用单光源、双光路结构,能够对测量信号和参考信号同时进行处理。采用所设计的筒式光纤探头激发并探测荧光,设计了相应的信号处理电路,实现了计算机管理。利用该系统和稳态光谱仪对西维因进行了对比实验。结果表明:在激发波长为319nm、荧光波长为654nm时,最小检测浓度为5×10-7μg/L。当西维因浓度范围在0.0～120.0μg/L之间时,系统具有较好的线性关系,线性相关系数r=0.9996(信噪比S/N=5)。该系统达到了荧光检测的指标。     

一种实现显微荧光寿命图的测量方法

将脉宽120fs、重复率76MHz激光引入激光扫描显微镜的激发光路,利用其扫描系统对荧光标记样品激发扫描,将激发出的荧光从荧光探测光路引入备用的外部探测口;在探测口接一快速光电倍增管,将光电倍增管的信号送给时间相关单光子计数器,获得时间相关的荧光强度图;最后通过计算机处理获得荧光寿命图。应用此系统对青色荧光蛋白(CFP)、黄色荧光蛋白(YFP)荧光寿命进行了测量,并应用CFP、YFP实现荧光共振能量转移的测量。通过实验看出利用已有的激光扫描显微镜,配合较先进的寿命测量方法,可以很好地实现显微荧光寿命图的测量。     

X-ray metrology for advanced silicon processes

X-ray reflectivity (XRR), X-ray fluorescence (XRF) and small angle X-ray scattering (SAXS) techniques are used to the monitoring of Cu/porous low κ processes, which are developed for the next generation (≤65 nm) integrated circuits. Sensitivity of XRR and XRF is sufficient to detect drifts of the copper barrier layer, copper seed layer and Cu CMP (chemical-mechanical polishing) processes. Their metrology key parameters comply with production requirements. SAXS allows determining the pore structure of low κ films: average pore size and pore size distribution.     

X射线荧光光谱检测多层薄膜样品的增强效应研究

研究了X射线荧光光谱检测多层薄膜样品的增强效应。根据多层膜中的X荧光强度理论计算公式编写了计算机程序,并计算了Zn/Fe和Fe/Zn双层膜样品中不同薄膜厚度时Fe Kα的一次荧光强度、二次荧光强度、二次荧光与一次荧光强度比以及二次荧光在总荧光强度中比例。研究发现,在多层膜样品的X射线荧光分析中,激发条件不变的情况下,元素谱线的一次荧光相对强度、二次荧光相对强度和二次荧光在总荧光强度中所占比例都随薄膜厚度及位置的变化而变化。当Fe和Zn层厚度相同时,随厚度的变化,对于Fe/Zn样品,Fe Kα二次荧光强度占总荧光强度最高为9％,而对于Zn/Fe样品这一比例最高可达35％。     

激光诱导水体频率上转换的荧光发射

用Nd：YAG的二倍频532 nm激光对几种不同水体的激光诱导荧光(LIF)光谱进行了测量,利用特征光谱荧光标记(SFS)技术指认出水体中溶解有机物(DOM)、叶绿素a(Chl a)及类胡萝卜素等物质的特征光谱带。指出在455 nm波长处具有较大强度的荧光峰是附属色素中抗氧化作用的类胡萝卜素(PPC)的贡献。提出了激光诱导PPC荧光频率上转换发射的动力学模型。     

Proposition of Single Molecular Orientation Determination Using polarization Controlled Beam by Liquid Crystal Spatial Light Modulators

We have proposed a method to control the three-dimensional electric field in the focus of an optical microscope using two non-twisted liquid crystal spatial light modulators, and to detect the molecular orientation of a single molecule. The three-dimensional electric field is generated by focusing the beam with two dimensional spatial distribution of polarization. The possibility of detection of three-dimensional single molecular orientation was shown by numerical calculations. © 2005 The Optical Society of Japan     

Finding of Optimal Calcium Ion Probes for Fluorescence Lifetime Measurement

We have investigated the fluorescence lifetime properties of 8 calcium ion probes, calcium-green-1, calcium green-2, calcium green-5N, calcium orange, oregon green 488 BAPTA-6F, fluo-3, fluo-4, and fluo-5N. We found that the decay time of calcium green-5N varied more sensitively with calcium concentration than calcium green-1 which was known to be a highly sensitive probe. We have also found that the center of observable range of calcium concentration by fluorescence lifetime measurement is lower than that by fluorescence intensity measurement.     

Effects of Refractive Index and Viscosity on Fluorescence and Anisotropy Decays of Enhanced Cyan and Yellow Fluorescent Proteins

The fluorescence lifetime strongly depends on the immediate environment of the fluorophore. Time-resolved fluorescence measurements of the enhanced forms of ECFP and EYFP in water–glycerol mixtures were performed to quantify the effects of the refractive index and viscosity on the fluorescence lifetimes of these proteins. The experimental data show for ECFP and EYFP two fluorescence lifetime components: one short lifetime of about 1 ns and a longer lifetime of about 3.7 ns of ECFP and for EYFP 3.4. The fluorescence of ECFP is very heterogeneous, which can be explained by the presence of two populations: a conformation (67% present) where the fluorophore is less quenched than in the other conformation (33% present). The fluorescence decay of EYFP is much more homogeneous and the amplitude of the short fluorescence lifetime is about 5%. The fluorescence anisotropy decays show that the rotational correlation time of both proteins scales with increasing viscosity of the solvent similarly as shown earlier for GFP. The rotational correlation times are identical for ECFP and EYFP, which can be expected since both proteins have the same shape and size. The only difference observed is the slightly lower initial anisotropy for ECFP as compared to the one of EYFP.