催化动力学荧光光度法测定痕量铜

在氨性介质中，铜对H2O2氧化次甲基蓝褪色反应有强烈催化作用。研究发现，次甲基蓝的氧化产物在紫外线照射下发出强荧光，据此建立一种测定痕量铜的催化动力学荧光光度法。本法检出限达0．02ng／mL，铜的质量浓度在0～6ng／mL范围内与相对荧光强度（△F）有良好线性关系。     

生物样品中Se的荧光测定方法

运用微波消化系统处理生物样品，以2，3-二氨基萘为荧光试剂建立了一种测定生物样品中Se的荧光分光光度法。方法的最低检出限为1．6ng／mL，线性范围0～0．600μg／mL，回收率92．22％～99．78％，连续10次测定样品变异系数（CV）为0．4％（n=10），隔213重复实验变异系数为1．54％。该法具有灵敏、稳定、可靠等优点，适用于生物样品中Se含量的测定。     

利用荧光共振能量转移体系测定食品中NO2-的研究

在λcx/λem=450／580nm，0．1mol／L的HCl溶液中，番红花红T和吖啶橙能够发生有效的共振能量转移，使得番红花红T荧光增强，同时吖啶橙的荧光猝灭，而NO2^-的加入使得两者的荧光强度同时减弱。由此建立了一种新的测定痕量NO2^-的方法。结果表明，NO2^-在0．02～10μg／mL范围内与染料的荧光强度减弱程度呈良好的线性关系，方法检出限为1．73ng／mL；该法用于食品中NO2^-的测定，回收率为105．0％～112．4％。     

微波消解-氢化物发生原子荧光光谱法同时测定化肥中砷、汞含量

采用微波消解样品前处理手段以及双道原子荧光光度计,建立了微波消解一氢化物发生原子荧光光谱法同时测定化肥中砷、汞含量的方法。通过试验确定了样品前处理方法,对负高压、灯电流,载气、屏蔽气、原子化器高度、酸度等测试条件进行了优化。在优化的工作条件下,砷、汞含量分别在0-50ng／mL和0—1．0ng／mL范围内与荧光强度呈良好的线性关系,线性相关系数分别为0．9996,0．9996,检出限分别为0．085,0．008ng／mL,回收率分别为88．8％～107．4％,90．0％～120％,测定结果的相对标准偏差均小于7％（n=6）。     

左旋氧氟沙星的荧光光谱法研究

提出了一种测定左旋氧氟沙星（LEV）的荧光光谱新方法。该法基于电子受体氯冉酸（CL）和2,3-二氰-5,6-二氯-1,4-对苯醌（DDQ）与电子给体左旋氧氟沙星之间的荷移反应,显示这两种受体能强烈增敏LEV的荧光强度。对影响反应的不同变量和参数进行了研究,建立了两种荧光光谱法测定LEV的新体系：（1）CL体系,线性范围为0．06～3．6μg／mL,检出限为0．02μg／mL;（2）DDQ体系,线性范围为0．12～2．2μg／mL,检出限为0．04μg／mL。所提方法已用于制剂中左旋氧氟沙星含量的测定,回收率分别为99．72％～99．36％和99．36％～98．86％。     

胶束增敏法测定盐酸左氧氟沙星的研究

研究了盐酸左氧氟沙星（OFLX）在胶束体系中的荧光性质，发现十二烷基硫酸钠对OFLX有较强的增敏作用，据此建立了胶束增敏荧光光谱法测定痕量OFLX的新方法。其线性范围为0～1．00μg/mL，检出限为4．73ng／mL。     

氢化物发生-原子荧光光谱法测定植物提取物中砷

建立了测定植物提取物中微量砷的原子荧光光谱方法,方法灵敏度高,准确度好。在选定的实验条件下,荧光强度与砷浓度在0～17ng／mL范围内成线性关系,相关系数0．9993,检出限0．4ng／mL,回收率92．3％～98．1％,相对标准偏差不超过4．2％。     

硫脲树脂富集-电感耦合等离子体质谱法测定地质样品中的超痕量金、银、铂、钯

研究了硫脲树脂富集，ICP-MS同时测定地质样品中超痕量金、银、铂、钯的方法。确定了仪器的最佳条件，并从吸附酸度、时间、树脂用量、解脱条件、干扰情况等方面进行了详细的考察。方法的检出限（3a）分别为Au：0．1lng／mL；Ag：0．35ng／mL；Pt：0．095ng／mL；Pd：0．08ng／mL。方法的RSD为（n=12）Au4．1％、Ag2．1％、Pt3．1％、Pd3．8％。测定了国家一级地球化学标准物质中的痕量Au、Ag、Pt、Pd，结果与标准值相吻合。     

DNA荧光探针—荧光素-中性红体系的研究

基于DNA对荧光素(FL)-中性红(NR)分子间荧光能量转移的抑制作用，以荧光素-中性红为荧光探针，考察该探针与DNA的结合反应，建立了准确测定DNA的新方法，在pH＝6.5条件下，hsDNA、ctDNA和smDNA的浓度与荧光素-中性红体系的荧光比值变化量Δ(Fd／Fa)成线性关系，响应线性范围分别为0．25-6．25μg／mL、0．10-5．00μg／mL、0．10-4．00μg／mL，0.025μg/mL和0．023μg／mL；分析测定了DNA合成样品，回收率91．3％-101．4％，相对标准偏差小于4．2％．     

氢化物-原子荧光光谱法测定面粉中的铅

利用AFS-920双道原子荧光光度计，采用氢化物-原子荧光法测定面粉中的铅含量，通过试验确定了仪器工作参数，载气、屏蔽气流量，介质和掩蔽剂的用量等。该法测定食品中铅含量的相对标准偏差为0.5％（n=11），检出限为0．1ng／mL。铅的浓度在0～40ng／mL与荧光强度呈线性关系，相关系数大于0.999。该法的加标回收率为95．0％～105．0％。     

Application of functionalized CdS nanoparticles as fluorescence probe in the determination of nucleic acids

Nanometer-sized fluorescent particles were successfully synthesized. The nanoparticles have a narrow, tunable, symmetric emission spectrum and a broad, continuous excitation spectrum. They are also photochemically stable. A synchronous fluorescence method was developed for the rapid determination of DNA with functionalized CdS as a fluorescence probe, based on the synchronous fluorescence quenching of functionalized CdS in the presence of DNA. Maximum fluorescence is produced at pH 7.0, with maximum excitation and emission wavelengths of 360 and 620 nm, respectively. The maximum emission wavelength of synchronous fluorescence is 354 nm when delta lambda = 260 nm. Under optimum conditions, the calibration graphs are linear over the range 0-3.5 microg mL(-1) for calf thymus DNA (CT-DNA) and 0.2-3.0 microg mL(-1) for fish sperm DNA. The corresponding detection limit is 0.01 microg mL(-1) for CT-DNA and 0.02 microg mL(-1) for fish sperm DNA. The relative standard deviation of seven replicate measurements is 2.2% for 1 microg mL(-1) calf thymus DNA and 2.4% for 1 microg mL(-1) fish sperm DNA. The method is simple, rapid and sensitive. The recovery and relative standard deviation are very satisfactory.     

Determination of nucleic acids by near-infrared fluorescence quenching of hydrophobic thiacyanine dye in the presence of Triton X-100.

A near-infrared (near-IR) fluorescence quenching method was developed for the determination of nucleic acids in aqueous solution by using a cationic heptamethylene thiacyanine as a probe. The near-IR cationic cyanine showed maximum excitation and emission wavelengths at 800 and 825 nm, respectively, in the presence of Triton X-100; the fluorescence of the cyanine could be greatly quenched by DNA. The calibration graphs were linear over the range of 10-400 ng/mL for CT (calf thymus) DNA and over the range 5-400 ng/mL for FS (fish sperm) DNA under optimal conditions. The corresponding detection limits were 5.2 ng/mL for CT DNA and 2.5 ng/mL for FS DNA. The relative standard deviation (n = 8) was 3.1% for 75 ng/mL CT DNA and 2.2% for 75 ng/mL FS DNA, respectively. Preliminary research showed that the fluorescence quenching might be ascribed to the formation of dye aggregate facilitated by DNA.     

Cationic cyanine as a near-infrared fluorescent probe for the determination of nucleic acids

A new method with a cationic near-IR cyanine as fluorescent probe was developed for the determination of nucleic acids. The near-IR cyanine shows maximum excitation and emission wavelengths at 765 and 790 nm, respectively, in aqueous solution. The method is based on the fluorescence decrease of near-IR cyanine in the presence of nucleic acids. Under optimal conditions, the ratio of fluorescence intensity in the absence and presence of nucleic acids was proportional to the concentration of nucleic acids over the range 0.10-1.2 microg/mL for CT (calf thymus) DNA or SM (salmon sperm) DNA, and 0.10-1.6 microg/mL for yeast RNA. The detection limits were 30 ng/mL for CT DNA, 25 ng/mL for SM DNA and 70 ng/mL for yeast RNA. The relative standard deviation (n = 6) was 2.1% for 500 ng/mL CT DNA, 2.4% for 500 ng/mL SM DNA and 2.7% for 500 ng/mL yeast RNA, respectively.     

Highly luminescent water-dispersed silicon quantum dots for fluorometric determination of oxytetracycline in milk samples

A fluorescent probe based on silicon quantum dots (SiQDs) was developed for the selective and sensitive detection of oxytetracycline (OTC) via the inner filter effect (IFE). The water-soluble fluorescent SiQD was synthesized based on the reaction of 3-Aminopropyltriethoxysilane (APTES) and sodium citrate as precursors by the one-pot hydrothermal process. The strong fluorescence emission of quantum dots (QDs) was obtained at 440 nm when excited at 350 nm and OTC had a broad absorption band between 200 and 400 nm. The excitation spectrum of SiQDs was completely overlapped with the absorption spectrum of OTC. The light at an excitation wavelength of QDs absorbed by OTC caused a decrease in fluorescence intensity with an increase in the concentration of OTC. Under optimal conditions, the linear concentration range was 0.92–9.2 µg mL1 with a detection limit (LOD; S/N = 3) of 0.19 µg mL ^-1 . The proposed method was applied to the determination of OTC in milk samples and satisfactory recoveries (98.8–100.5%) with low RSD % values (0.93–2.31%) were achieved. This simple, selective, sensitive, rapid, and cheap method can be used as a promising tool for OTC analysis in food safety.     

紫外-可见吸收光谱和荧光光谱研究壳核型 CdTe/CdS量子点与盐酸巴马汀的相互作用及其分析应用

合成了巯基乙酸(TGA)修饰的壳核型CdTe/CdS量子点(TGA-CdTe/CdS QDs), 利用紫外-可见光谱和荧光光谱研究了TGA-CdTe/CdS QDs与盐酸巴马汀(PC)的相互作用机理. 结果表明, 在pH=7.4的Tris-HCl缓冲液中, QDs与PC相互作用后使QDs的荧光呈线性猝灭, 并有良好的线性关系(r=0.997), 线性范围为25~1×10⁴ ng/mL, 检出限(3σ)为7.7 ng/mL. 建立了一种快速简便、 可定量测定PC的新方法.     

Cationic cyanine as a near-infrared fluorescent probe for the determination of nucleic acids

A new method with a cationic near-IR cyanine as fluorescent probe was developed for the determination of nucleic acids. The near-IR cyanine shows maximum excitation and emission wavelengths at 765 and 790 nm, respectively, in aqueous solution. The method is based on the fluorescence decrease of near-IR cyanine in the presence of nucleic acids. Under optimal conditions, the ratio of fluorescence intensity in the absence and presence of nucleic acids was proportional to the concentration of ¶nucleic acids over the range 0.10–1.2 μg/mL for CT (calf thymus) DNA or SM (salmon sperm) DNA, and 0.10–¶1.6 μg/mL for yeast RNA. The detection limits were ¶30 ng/mL for CT DNA, 25 ng/mL for SM DNA and ¶70 ng/mL for yeast RNA. The relative standard deviation (n = 6) was 2.1% for 500 ng/mL CT DNA, 2.4% for ¶500 ng/mL SM DNA and 2.7% for 500 ng/mL yeast RNA, respectively.     

Determination of Plumbagin in Plant Extracts and Polyherbal Formulations by High-Performance Liquid Chromatography with Fluorescence Detection

Plumbagin, a naturally occurring naphthoquinone derivative, is known to possess various pharmacological activities. A rapid, sensitive, and specific high-performance liquid chromatographic method using fluorescence detection is reported for the determination of plumbagin in two Plumbago species and five polyherbal formulations. The method employed a reverse phase C18 column with isocratic elution using 65:35 pH 3.2 methanol and 0.1% aqueous o-phosphoric acid at a flow rate of 1.0 mL/min. Plumbagin displayed maximal fluorescence with excitation at 264 nm and emission at 605 nm. A linear calibration relationship was obtained for 1 to 10 µg/mL plumbagin with limits of detection and quantitation of 8 ng/mL and 30 ng/mL, respectively. The relative standard deviation values for intraday and interday precision were less than 2%. The recoveries were greater than 97% with relative standard deviations less than 3%. This is the first study to employ high-performance liquid chromatography with fluorescence detection for the determination of plumbagin. The method was rapid, sensitive, and accurate for the analysis of plants and polyherbal formulations.     

Determination of nucleic acids using calcein-neodymium complex as a fluorescence probe.

A novel fluorometric method has been developed for rapid determination of DNA and RNA with calcein-neodymium complex as a fluorescence probe. The method is based on the fluorescence enhancement of calcein-Nd(III) complex in the presence of DNA or RNA, with maximum excitation and emission wavelength at 489 nm and 514 nm, respectively. Under optimal conditions, the calibration graphs are linear over the range 0.5 - 3.0 microg/ml for both DNA and yeast RNA, 0.4 - 2.0 microg/ml for fish sperm DNA (FS DNA) and 0 - 3.0 microg/ml for calf thymus DNA (CT DNA). The corresponding detection limits are 15.1 ng/ml for DNA, 21.2 ng/ml for yeast RNA, 10.5 ng/ml for FS DNA and 8.9 ng/ml for CT DNA. The interaction mechanism for the binding of calcein-Nd(III) complex to DNA is also studied. The results of absorption spectra, fluorescence polarization measurements and thermal denaturation experiments, suggested that the interaction between calcein-Nd(III) complex and DNA is an electrostatic interaction.     

水溶性发光金量子点灵敏检测L-半胱氨酸

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0~4.0 μmol/L浓度范围内呈线性关系,线性相关系数R2=0.9976,对2.0 μmol/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。     

基于BHHCT-Eu3+@SiO2荧光稀土二氧化硅纳米颗粒的免疫层析试纸条检测卡那霉素

采用微波辅助合成的荧光稀土二氧化硅纳米颗粒(BHHCT-Eu3+@SiO2)为标记物,建立了快速定量检测卡那霉素(Kana)残留的荧光免疫层析方法.实验结果表明,微波辅助合成的BHHCT-Eu3+@SiO2纳米颗粒呈球形,粒径约36 nm,具有良好的荧光发射性能,最大吸收波长和最大发射波长分别为343和615 nm.将BHHCT-Eu3+@SiO2与卡那霉素抗体(Kana-ab)通过醛基化葡聚糖交联,合成了荧光标记抗体Eu3+-Kana-ab,结合定量侧向层析读数仪,建立了牛奶中Kana残留的快速定量检测方法,对Kana的检出限(IC10)为0.85 ng/mL,半数抑制浓度(IC50)为12.76 ng/mL,检测范围(IC20-IC80)为3.0~76.0 ng/mL,牛奶中的Kana的加标回收率范围为93.7%~97.4%,RSD为3.1%~4.6%,与Kana类似物的交叉反应均<1%.牛奶中Kana残留的测定结果与ELISA方法相关性良好.