某些蒽环类抗癌药物与刚果红相互作用的吸收、荧光和共振瑞利散射光谱研究

在pH 2.5左右的酸性介质中, 刚果红与表柔比星、柔红霉素和米托蒽醌等蒽环类抗生素反应形成离子缔合物时, 仅能引起吸收光谱和荧光光谱的微小变化, 但却能导致共振瑞利散射(RRS)的显著增强并产生新的RRS光谱, 与此同时也观察到二级散射(SOS)和倍频散射(FDS)的增强. 最大RRS峰位于370 nm附近, 并在280 nm附近有另一散射峰. 而它们的SOS峰均在530 nm附近, 最大FDS峰均位于353 nm处. 其中RRS法灵敏度最高, 它对表柔比星、柔红霉素和米托蒽醌的检出限分别为0.054, 0.058和0.033 μg/mL, 而其线性范围分别为0.05～12.0, 0.05～12.0和0.04～7.5 μg/mL. 文中研究了反应产物的吸收、荧光和RRS光谱特征, 适宜的反应条件及分析化学性质, 据此发展了一种用RRS技术灵敏、简便、快速测定蒽环类抗癌药物的新方法.     

Resonance Rayleigh scattering measurement of aminoglycoside antibiotics with Evans Blue.

In a weak acid medium, some aminoglycoside antibiotics, such as kanamycin (KANA), gentamicin (GEN), tobramycin (TOB) and neomycin (NEO), or acid bisazo dye Evans Blue (EB) can only produce very weak resonance Rayleigh scattering (RRS) signals. However, when two agents react with each other to form ion-association complexes, the RRS intensity can be greatly enhanced and a new RRS spectrum with a significant enhancement of the RRS intensity in the wavelength range from 350 nm to 600 nm can be observed. The maximum scattering peak is at 570 nm. There is a linear relationship between the RRS intensity and the antibiotic concentration in the range of 0.01-6.0 microg mL(-1) at 570 nm. This RRS method for the determination of aminoglycoside antibiotics at trace-amount levels has been developed. The detection limits (3sigma) of the four antibiotics, whose order of sensitivity from high to low ranks as KANA > NEO > TOB > GEN, are 5.2-6.9 ng mL(-1). This method has good selectivity and has been successfully applied to the quick determination of antibiotics not only for injections and ear drops, but for clinic serum samples as well. In addition, the reaction mechanism by using a quantum chemistry method and the influencing factors of the RRS spectra and the enhancement reasons of RRS have been discussed.     

Determination of Matrine and Oxymatrine in Radix Sophorae Flavescentis by Resonance Rayleigh Scattering,Second-order Scattering and Frequency Doubling Scattering Technique

In 0.1 mol/L HCl medium, 12-tungstophosphoric(TP) acid reacted with matrine(Mat) and oxymatrine(Oxy) to form an ion-association complex. As a result, the new spectra of resonance Rayleigh scattering(RRS), second-order scattering(SOS) and frequency doubling scattering(FDS) appeared and their intensities were enhanced greatly. The maximum scattering wavelengths of RRS, SOS and FDS were located at 370, 670 and 390 nm, respectively. The increments of scattering intensity were directly proportional to the concentration of Mat and Oxy in a certain range. Based on this, the method for the determination of matrine and oxymatrine has been established. It has been applied to the determination of matrine and oxymatrine in samples of Radix sophorae flavescentis with satisfactory result. The reaction mechanism and reasons of RRS enhancement were discussed.     

Resonance Rayleigh scattering study of the interaction of bleomycinA_5 with nucleic acids and its analytical application

The interaction of bleomycinA5 with nucleic acids has been investigated by using resonance Rayleigh scattering (RRS), molecular absorption and fluorescence spectra. The result shows that in near pH 2.2 buffer medium and absence of any metal ions, nucleic acids are capable of binding with bleomycinA5 (BLMA5) to form complexes which can remarkably enhance the RRS intensity and result in batho- chromic and hyperchromic molecular absorption of nucleic acids and fluorescence quenching of bleomycinA5. The RRS spectral characteristics for the binding products of bleomycinA5 with various DNA and RNA are similar, and the maximum RRS peaks are at 301 nm for ctDNA and sDNA, 370 nm for hsDNA, 310 nm for RNAtypeVI and RNAtypeIII, respectively. The increments of RRS intensity are greatly different in which DNA enhances greatly and RNA enhances lightly. In this work, the optimum condi- tions of the interaction and some influencing factors have been investigated. The reaction mechanism and a binding model for the interaction of BLMA5 with the nucleic acids are discussed. In addition, a highly sensitive, simple and rapid new method for the determination of DNA has been developed. The detection limits (3σ) are 5.7 ng/mL for ctDNA, 7.4 ng/mL for sDNA and 9.2 ng/mL for hsDNA, respectively. The method can be applied to determination of trace amounts of DNA.     

Resonance Rayleigh scattering spectra for studying the interaction of aminoglycoside antibiotics with pontamine sky blue and their analytical applications

In a weakly acid medium, some aminoglycoside antibiotics, such as kanamycin (KANA), gentamicin (GEN), tobramycin (TOB), and neomycin (NEO), or acid bisazo dye pontamine sky blue (PSB) can only produce very weak resonance Rayleigh scattering (RRS) signals. However, when the two agents react with each other to form the ion association complexes, the RRS intensity can be enhanced greatly and a new RRS spectrum and a significant enhancement of the RRS intensity in the wavelength range 350-600 nm can be observed. The maximum scattering peak is at 580 nm. There is a linear relationship between the RRS intensity and the antibiotic concentration in the range 0.01-6.0 microg mL(-1) at 580 nm. This RRS method has therefore been developed for the determination of trace levels of aminoglycoside antibiotics. The detection limits (3 sigma) of the four antibiotics, whose order of sensitivity is KANA>NEO>TOB>GEN, are 5.8-6.9 ng mL(-1). This method has a good selectivity and has been successfully applied to the quick determination of antibiotics not only for injections and ear drops, but clinic serum samples as well. In addition, quantum chemistry-based analysis of the reaction mechanism, the factors influencing the RRS spectra, and the reasons for the enhancement of RRS are discussed.     

甲基紫硫酸软骨素共振瑞利散射光谱及其应用

在Britton-Robinson缓冲介质(pH9.37)中硫酸软骨素与甲基紫反应形成离子缔合物时,共振瑞利散射(RRS)强度会明显增强,其最大RRS峰位于505和661 nm处。本文对反应的最佳条件、影响因素、硫酸软骨素浓度与RRS强度的关系进行了研究,建立起一种快速、简便、灵敏的测定硫酸软骨素的方法。本法在661和505 nm测定波长处的线性范围均为:0.15~0.90 mg/L,其检出限分别为0.019 mg/L(505 nm)和0.043mg/L(661 nm)。该法应用于针剂中硫酸软骨素的测定,结果满意。     

曲利本红与氨基糖苷类抗生素相互作用的共振瑞利散射光谱及其分析应用

在弱酸条件下，酸性双偶氮染料曲利本红（TR）或硫酸卡那霉（KANA）、硫酸 新霉素（NEO）、硫酸庆大霉素（GEN）和硫酸妥布霉素（TOB）等氨基糖苷类抗生 素的各自共振瑞利散射（RRS）十分微弱，但两者相互作用形成离子缔合物时能使 RRS急剧提高并产生新的RRS光谱，在400～535nm之间有一个强的散射带，最大散射 峰位于400nm处，在0.013～6.0μg·mL~(-1)范围内RRS强度与抗生素浓度成正比， 可用于氨基糖苷类抗生素的测定，对不同抗生素的检出限（3σ）在12.9～17.6ng ·mL~(-1)之间，其灵敏度的顺序是KANA＞NEO＞TOB＞GEN,方法有较好的选择性， 可用于市售抗生素注射液或滴耳液中药物含量和临床血药浓度的快速测定，中还用 量子化学方法对反应机理进行探讨，并讨论了的RRS光谱特性的影响因素和RRS增强 的原因。     

同多钨酸-阿米卡星相互作用的共振瑞利散射光谱及其分析应用

在pH 0.65~1.10的HCl-NaAc缓冲溶液中,当同多钨酸(IPT)与阿米卡星(AMK)形成离子缔合物,能引起共振瑞利散射 (RRS)显著增强,并产生新的RRS光谱,其最大散射峰位于340 nm,AMK浓度在0.001~0.08 µg•mL-1范围内与散射增强程度呈线性关系,据此建立测定AMK的RRS新方法。方法具有较高的灵敏度,检出限(3σ)为0.4 ng•mL-1。考察了体系的RRS和吸收光谱特征,优化了适宜的反应条件,试验了常见共存物质的影响,表明方法具有良好的选择性。方法用于人血清中AMK的测定,结果满意。文中对离子缔合反应机理和RRS增强的原因进行了讨论。     

固绿FCF共振瑞利散射法测定食品中的Al(Ⅲ)

在酸性Tris-HCl缓冲介质中,溴化十六烷基三甲基铵(CTMAB)增敏固绿FCF,与Al(Ⅲ)结合生成三元络合物使共振瑞利散射(RRS)显著增强并产生新的RRS光谱,其最大共振瑞利散射峰位于330 nm,RRS增强程度(△IRRS)与Al(Ⅲ)的质量浓度在0.02～0.49 mg/L成正比,方法有很高的灵敏度,检出限是0.0096 mg/L.方法用于面制食品中Al(Ⅲ)的测定,结果满意.     

金纳米微粒作探针共振瑞利散射光谱法测定盐酸异丙嗪

在pH 1.8～3.0的酸性介质中,质子化的盐酸异丙嗪(PMZ)可与带负电荷的金纳米微粒依靠静电和疏水作用相互结合,导致共振瑞利散射(RRS)强度显著增强,其最大散射峰位于368 nm,并在284,440,498 nm处有明显的散射峰,在选定的测量波长下,盐酸异丙嗪在0.04～0.10μg/mL的浓度范围内与RRS强度成正比,该法具有高的灵敏度,其检出限为1.34 ng/mL。考察了体系的RRS光谱特征,研究了适宜的反应条件、影响因素,研究了共存物质的影响,据此建立了金纳米微粒作探针RRS法测定盐酸异丙嗪的新方法。     

Resonance Rayleigh scattering study of the interaction of bleomycinA<Subscript>5</Subscript> with nucleic acids and its analytical application

The interaction of bleomycinA5 with nucleic acids has been investigated by using resonance Rayleigh scattering (RRS), molecular absorption and fluorescence spectra. The result shows that in near pH 2.2 buffer medium and absence of any metal ions, nucleic acids are capable of binding with bleomycinA5 (BLMA5) to form complexes which can remarkably enhance the RRS intensity and result in bathochromic and hyperchromic molecular absorption of nucleic acids and fluorescence quenching of bleomycinA5. The RRS spectral characteristics for the binding products of bleomycinA5 with various DNA and RNA are similar, and the maximum RRS peaks are at 301 nm for ctDNA and sDNA, 370 nm for hsDNA, 310 nm for RNAtypeVI and RNAtypeIII, respectively. The increments of RRS intensity are greatly different in which DNA enhances greatly and RNA enhances lightly. In this work, the optimum conditions of the interaction and some influencing factors have been investigated. The reaction mechanism and a binding model for the interaction of BLMA5 with the nucleic acids are discussed. In addition, a highly sensitive, simple and rapid new method for the determination of DNA has been developed. The detection limits (3σ) are 5.7 ng/mL for ctDNA, 7.4 ng/mL for sDNA and 9.2 ng/mL for hsDNA, respectively. The method can be applied to determination of trace amounts of DNA.     

盐酸表柔比星与核酸相互作用的共振瑞利散射光谱研究及其分析应用

用共振瑞利散射光谱研究了盐酸表柔比星(EPI)与小牛胸腺DNA(ctDNA)、鲑鱼DNA(sDNA)、鲱鱼精DNA(hsDNA)和酵母RNA(yRNA)等核酸之间的相互作用. 实验表明在pH 2.0左右的酸性介质中, 表柔比星及核酸本身的共振瑞利散射(RRS)均十分微弱, 但是当它们相互作用形成结合产物时, 将导致RRS增强并出现新RRS光谱. 不同核酸与表柔比星结合产物的RRS 光谱特征略有差异, 散射增强程度则各不相同, 其相对散射强度的顺序是ctDNA≈sDNA＞hsDNA＞yRNA . 在一定范围内核酸浓度与散射强度成正比, 据此可以建立一种新的用表柔比星测定DNA的 RRS 法, 方法具有高灵敏度, 对于不同DNA 其检出限(3s)在24.0 ng/mL 至28.0 ng/mL 之间, 用于合成样品分析, 结果满意. 文中还研究了适宜的反应条件, 影响因素和结合产物的分析化学性质. 结合吸收光谱和荧光光谱特征对表柔比星与DNA 的反应机理进行了讨论.     

共振瑞利散射光谱法对盐酸异丙嗪与盐酸氯丙嗪的同时测定

钼酸铵(AM)与盐酸氯丙嗪(CPZ)及盐酸异丙嗪(PZ)均能反应形成离子缔合物,引起共振瑞利散射(RRS)的显著增强,并出现新RRS光谱.2种反应产物具有相似的RRS光谱特征,其最大散射峰均在365 nm处,且在一定范围内散射增强(Δ_(IRRS))与药物的质量浓度成正比,但RRS强度随药物质量浓度的线性增幅存在显著差异.结合两组分RRS光谱强度的加和性,可建立双组分信号响应的两条同原射线的计量分析法.方法对CPZ 和PZ的检出限分别为4.5、7.7 μg/L,线性范围均为0.03～2.4 mg/L.将该方法用于血清、尿样和非那根止咳糖浆中CPZ和PZ的同时测定,取得满意结果.     

Resonance Rayleigh scattering spectrum for the chelate of lanthanum(Ⅲ) with sodium tanshinon ⅡA silate and its analytical application

In a pH 3.6-5.0 Hac-NaAc buffer solution, when sodium tanshinon ⅡA silate (STSⅡA) reacts with La(Ⅲ) to form a chelate, the resonance Rayleigh scattering (RRS) intensity can be enhanced greatly and a new RRS spectrum will appear. The maximum RRS peak is located at 306 nm and the RRS intensity is proportional to the concentration of STSⅡA in a certain range. The method is very sensitive and the detection limit for STSⅡA (3σ/K) is 82.12 ng·mL-1. The optimum reaction conditions and the effect of coexisting substances have been investigated. A new, simple and fast method for the determination of STSⅡA based on RRS method is developed. It can be applied to the determination of STSⅡA in the synthesis samples and Nuoxinkang injection. Combined with infrared absorption and NMR spectra, the structure of the chelate and the reasons of RRS enhancement are also discussed.     

共振瑞利散射法测定微量硒

在稀HCl中硒(Ⅳ)与抗坏血酸(Vc)反应生成单质硒Se(0),并在液相中以纳米粒子的形式存在。利用此纳米粒子在470nm处的共振瑞利散射峰可对硒进行测定。在0.028~5.640μg/mL范围内,共振瑞利散射强度与硒(Ⅳ)的质量浓度成线性关系,检出限为0.00789μg/mL,相对标准偏差为4.7%。应用此法测定了茶叶、螺旋藻、黄芪样品中的总硒量,通过与例行方法DAN荧光法对照、干扰实验、回收率实验及质量控制对本方法进行了评价。     

Ag(Ⅰ)-呋塞米相互作用的共振瑞利散射、二级散射和倍频散射光谱及其分析应用

在pH=3.5的HAc-NaAc介质中,呋塞米(FUR)与Ag(Ⅰ)形成1:1(摩尔比)的螯合物,从而引起共振瑞利散射(RRS)、二级散射(SOS)和倍频散射(FDS)光谱显著增强,其最大RRS,SOS和FDS波长分别位于310,584和330 nm.在一定范围内,3种散射信号的增强(△ⅠRRs,△ⅠSOS和△ⅠFDS...     

Resonance Rayleigh method for the determination of proteins with Orange G.

In pH 0.6 - 2.0 HCl-sodium acetate buffer solution, proteins react with an acidic monoazo dye such as Orange G, Methyl Orange, Methyl Red and Orange IV to form a combination product. This results in a significant enhancement of resonance Rayleigh scattering (RRS) and a new RRS spectrum appears. Owing to the fact that Orange G-protein system is the most sensitive, it was taken as an example to study. The RRS spectral characteristics of its combination product and the optimum condition for the reaction were investigated. The intensity of RRS is directly proportional to the concentration of protein in the range of 0 - 5.0 microg/mL. The method has high sensitivity; its detection limits are 2.6 ng/mL for BSA, 3.4 ng/mL for HAS and 7.1 ng/mL for alpha-chymotrypsin, respectively. A new method for the determination of trace amounts of proteins on the basis of RRS spectra has been developed.     

A new method for the determination of the critical micelle concentration of Triton X-100 in the absence and presence of beta-cyclodextrin by resonance Rayleigh scattering technology

A new method for the determination of the critical micelle concentration (CMC) of Triton X-100 in aqueous solution and beta-cyclodextrin solution by resonance Rayleigh scattering (RRS) has been developed. The method is based on the measurement of the RRS intensity of different concentration of Triton X-100 in aqueous solution and beta-cyclodextrin solution (6.0 x 10(-4) mol l(-1)). When the RRS intensities were plotted against the concentration of Triton X-100, an inflection point appeared at the Triton X-100 concentration of 5.0 x 10(-4) mol l(-1) in aqueous solution and 1.1 x 10(-3) mol l(-1) in beta-cyclodextrin solution, respectively. These values of concentration corresponded to the CMC of Triton X-100 in aqueous solution and beta-cyclodextrin solution, which also agreed closely with the results reported by surface tension and UV-Vis absorption spectrophotometry. Therefore, the present RRS method is very convenient, rapid and accurate and can be used as a new technology for the determination of CMC values of surfactants without any probe. The relationship between the RRS intensity and the concentration, aggregate state and the aggregate molecular size of Triton X-100 has been primarily discussed.     

利福霉素类抗生素-Cu(II)-核酸体系的RRS光谱研究

在Britton-Robinson (B-R)缓冲溶液中, 利福霉素类药物与ctDNA反应的适宜的pH范围是1.9～2.1. 此类药物本身有微弱RRS峰, 它们具有相似的光谱特征, 其散射峰均在290和370 nm附近; 而ctDNA的RRS峰在310 nm处. 两者反应形成结合产物后其RRS明显增强, 并在375 nm左右出现最大散射峰, 且有不同程度的红移和散射增强, 说明两者结合成新的产物; 加入Cu2＋离子后, Cu2＋与利福霉素抗生素及DNA形成三元复合物, 此时将导致RRS进一步剧增, 而且RRS光谱增强值与DNA浓度呈正比, 因而可用于DNA测定具有较高的灵敏度, 实验对ctDNA的检出限为9.7 ng/mL (RFSV-Cu2＋- ctDNA体系). 文中研究了三元配合物反应的适宜条件和影响因素, 基于此反应发展了一种用RRS技术测定DNA的新方法.     

胰蛋白酶与DNA相互作用的共振瑞利散射光谱及其分析应用研究

当胰蛋白酶与鲱鱼精DNA(hsDNA)、 鲑鱼精DNA(sDNA)以及小牛胸腺DNA(ctDNA)之间发生相互作用时,共振瑞利散射(RRS)会显著增强,并产生新的RRS光谱. 三者有近似的光谱特征,其最大RRS峰分别位于307 nm(hsDNA和sDNA体系)和290 nm处(ctDNA体系),另一散射峰位于350 nm处,其散射强度(ΔI)与DNA或者胰蛋白酶的浓度成正比,因此可用于蛋白质和DNA的相互测定. 当用胰蛋白酶测定DNA时,hsDNA,sDNA和ctDNA的检测范围分别为1.4×10^-3～2.3, 2.1×10^-3～2.5和3.5×10^-3～1.9 μg/mL(ctDNA),它们的检出限分别为0.4,0.7和1.1 ng/mL. 当用hsDNA测定胰蛋白酶时,其线性范围为0.1～30.0 μg/mL,检出限为39.0 ng/mL. 研究了最佳的反应条件、 影响因素和结合产物的化学性质,考察了胰蛋白酶与DNA的结合比,推测了它们的结合方式,并以胰蛋白酶作RRS探针,发展了一种高灵敏、 简便和快速测定痕量DNA的新方法.