共振光散射光谱的校正

以罗丹明6G在pH7.40时的共振光散射光谱（RLS）为例,引进仪器特性因子和分子吸收因子讨论荧光分光光度计的检测灵敏度和体系分子吸收对RLS光谱的影响,提出光谱校正方程。在吸收体系中,吸收带附近的散射光强度降低,并导致散射光谱发生畸变。通过光谱校正,除消除了不同仪器因光源和检测系统的差异对RLS光谱特性影响外,有效地消除了分子吸收的影响,提高了测定灵敏度。     

曙红Y的共振光散射与共振荧光

研究了曙红Y（EY）的共振散射光谱、荧光光谱和吸收光谱,讨论了共振光散射与共振荧光的区别与联系。在EY水溶液三维荧光等高线光谱图中,瑞利散射线与荧光等高线有部分相交。EY的共振散射峰（525nm）介于荧光激发峰（514nm）和发射峰（536nm）之间。由光偏振实验,测得EY共振散射光谱525nm处的偏振度P=0．20。上述实验结果证明,EY的共振散射峰主要是共振荧光。在改变pH的实验中发现,EY共振光散射增强是由于酸碱平衡的移动导致荧光型体的形成。由于自吸收的影响,共振散射光强度与EY浓度之间不是严格的线性关系。     

乙二醇中铜胶体共振光散射光谱

在乙二醇中,以聚乙烯吡咯烷酮（PVP）为分散剂,抗坏血酸（VC）为还原剂和抗氧化剂,还原CuSO4制得铜胶体溶液。 通过XRD、UV-Vis与共振光散射（RLS）光谱对铜胶体进行表征。 结果表明,铜胶体为面心立方晶体结构的0价铜,在592~602 nm呈现典型的等离子共振吸收峰,体系具有明显的RLS特征,最大散射波长在468 nm。 考察了反应条件、体系的稳定性与共存离子对乙二醇中铜胶体RLS的影响。 结果表明,适宜的反应条件为：试剂按照VC、CuSO4和PVP的加入顺序,3种物质量的比按照n(VC)/n(Cu2+)=15、n(PVP-K30)/n(Cu2+)=1.4;反应温度60 ℃;反应时间1 h,反应得到的铜胶体可稳定放置1 d。 在适宜条件下,ρ(Cu2+)在5.12~12.8 mg/L范围内与散射光强度（ΔIRLS）成正比,回归方程为ΔI=7 420.2ρ-631.8（r=0.9962）,检出限（3σ）为0.63 μg/L。 0.64 mg/L MnSO4、CdSO4和ZnSO4,1.28 mg/L KI,64 mg/L Na2CO3和Ca(OH)2,960 mg/L CH3CH2OH,640 mg/L CH3OH和320 mg/L CH3CH2CH2OH均不干扰10 mg/L Cu2+溶液的测量。 由此建立一种利用RLS光谱测定乙二醇中铜离子的简便方法。     

Resonance light scattering technique used for biochemical and pharmaceutical analysis

By coupling and scanning simultaneously excitation and the emission monochromators of a common spectrofluorometer, enhanced resonance light scattering (RLS) signals could be obtained. The enhanced RLS signals could be used for designating bio-assemblies, aggregation species, and analytical purposes. Herein, we review the reports since the year of 2000 concerning the biochemical and pharmaceutical analysis with the RLS measurements, and discuss the possible developments of this technique.     

Resonance light scattering spectroscopy study of interaction between norfloxacin and calf thymus DNA and its analytical application

The interaction between norfloxacin and calf thymus double-stranded DNA (dsDNA) has been studied by a resonance light scattering (RLS) technique with a common spectrofluorometer. The characteristics of RLS spectra, the effective factors and optimum conditions of the reaction have been investigated. In Britton-Robinson (BR) buffer (pH 5.87), norfloxacin has a maximum peak 405.5 nm and the RLS intensity is remarkably enhanced by trace amount of calf thymus dsDNA due to the interaction between norfloxacin and dsDNA. The binding of norfloxacin to DNA forms large particles, which were characterized by RLS spectrum, scanning electron microscopy (SEM), ultraviolet-visible (UV-vis) spectrum, and fluorescence spectrum. Based on the enhanced RLS intensity, a novel method for sensitive determination of calf thymus dsDNA concentration ranging from 0.02 to 2.3 microg ml(-1) was developed. The determination limit (3 sigma) was 1.2 ng ml(-1). The method is simple, rapid, practical and relatively free from interference generated by coexisting substance, as well as much more sensitive than most of the reported methods. Three synthetic samples of ctDNA were determined with satisfactory results.     

甲基紫与苋菜红相互作用的双波长共振光散射比率光谱研究及其分析应用

应用双波长共振光散射比率法(DW-RLS)研究了甲基紫与苋菜红之间的相互作用.在pH 1.24的乙酸钠-HCl缓冲溶液中,甲基紫和苋菜红本身的共振光散射(RLS)信号均很弱,但是当它们相互作用形成缔合物时,导致RLS信号明显增强并出现新的RLS光谱,适当浓度的Triton X-100存在使结合反应敏化,缔合物最大散射峰位于528 nm,RLS信号强度与苋菜红的浓度呈线性关系.通过测量528 nm处的RLS强度或两个波长处RLS强度比值(I417/I343),可对苋菜红进行定量检测.当溶液中甲基紫的浓度为1.54×10-5 mol/L时,RLS法测定苋菜红的线性范围和检出限分别为0.05～0.50 μg/mL和0.02 μg/mL,而DW-RLS法的线性范围和检出限分别为0.01～0.60 μg/mL和1 ng/mL,与RLS法相比较,DW-RLS法受酸度、离子强度等环境条件影响较小,并且有更宽的线性范围和更低的检出限.     

盐酸奎宁与全氟辛烷磺酸体系的共振光散射光谱研究及其分析应用

研究了盐酸奎宁(Quinine dihydrochloride,简称Quinine)与全氟辛烷磺酸(perfluorooctane sulfonate,简称PFOS)相互作用的共振光散射(resonance light scattering,RLS)光谱,并建立了PFOS的共振光散射分析方法.在pH值为2.87的Britton-Robinson(BR)缓冲溶液中,全氟辛烷磺酸根阴离子与质子化的盐酸奎宁通过静电引力和疏水作用形成2:1的离子缔合物,引起共振光散射强度(IRLS)显著增强,最大散射波长位于283nm处,增强的散射信号强度与PFOS浓度在0.10～50.0μmol/L范围内呈线性关系,据此建立了测定PFOS的散射分析方法,检测限为9.88nmol/L.讨论了体系的最佳反应条件及外来物质的干扰,同时研究了体系的吸收光谱及荧光光谱,并探讨了反应机理.本方法用于水样及人体血清样品中PFOS的测定,RSD≤4.2%.     

结晶紫共振光散射法测定脱氧核糖核酸

研究了三苯甲烷类碱性染料结晶此与DNA作用的共振光散射光谱,在pH9.2-10.5的范围内,加入DNA导致结晶紫共振光散射增强,在512nm处,存在一共振光散射增强峰,其强度与DNA的浓度呈线性关系,据此建立了一种测定DNA的菜振光散射法,方法的线性范围为0－900ng/mL,检出限为5.02mg/mL.已用于混合样品中的DNA的测定.     

Microdetermination of proteins using m-carboxychlorophosphonazo as detection probe by enhanced resonance light scattering spectroscopy

Proteins can be determined using a common spectrofluorometer to detect the intensity of resonance light scattering (RLS). Under acidic conditions, the reaction between m-carboxychlorophosphonazo (CPA-mK) and proteins enhances the weak light scattering of CPA-mK drastically. This enhanced intensity is proportional to the concentration of proteins. The linear ranges for human serum albumin are 0.5-35.0 microg/mL, with detection limits of 0.104 microg/mL. The method yields results comparable to those of the calorimetric method using Coomassie Brilliant Blue G-250 (CBB) with relative standard deviations of 0.72-2.10% (n = 10). There is almost no interference by amino acids and most of the metal ions.     

Study on the toxic interaction of methanol, ethanol and propanol against the bovine hemoglobin (BHb) on molecular level

The toxic interaction of methanol, ethanol and propanol with bovine hemoglobin (BHb) at protein molecular level was studied by resonance light scattering (RLS), fluorescence, ultraviolet-visible absorption (UV-vis) and circular dichroism (CD) techniques. The experimental results showed that the three alcohols all had toxic effects on BHb and the effects increased along with the increasing alcohol dose. The results of RLS and fluorescence spectroscopy showed that alcohols can denature BHb. They changed the microenvironment of amino acid residues and led to molecular aggregation. The decreasing order of the influence is propanol, ethanol and methanol. The results of UV-vis and CD spectra revealed that alcohols led to conformational changes of BHb, including the loosening of the skeleton structure and the decreasing of α-helix in the second structure. The changes generated by propanol were much larger than those by methanol and ethanol.     

Study on the interaction between a fluorine-containing amphiphilic cationic copolymer and nucleic acid by resonance light scattering technique

A novel fluorine-containing amphiphilic cationic copolymer P(HFMA-St-MOTAC)-g-PEG was synthesized as a new probe to detect DNA based on the RLS technique. The aggregation of P(HFMA-St-MOTAC)-g-PEG on the molecular surface of DNA occurred under pH 4.0-7.0 resulted in an enhanced resonance light-scattering (RLS) peaks at 370 nm, 400 nm, 420 nm and 470 nm. The intensity of resonance light-scattering was found to be proportional to the concentration of DNA. The detection limit was 5.8 μg L⁻¹. It was found that the P(HFMA-St-MOTAC)-g-PEG has strong interaction with DNA as confirmed by the resonance light scattering (RLS) spectroscopy, UV spectra, IR spectra, and TEM.     

Microdetermination of proteins using m-carboxychlorophosphonazo as detection probe by enhanced resonance light scattering spectroscopy

Proteins can be determined using a common spectrofluorometer to detect the intensity of resonance light scattering (RLS). Under acidic conditions, the reaction between m-carboxychlorophosphonazo (CPA-mK) and proteins enhances the weak light scattering of CPA-mK drastically. This enhanced intensity is proportional to the concentration of proteins. The linear ranges for human serum albumin are 0.5–35.0 μg/mL, with detection limits of 0.104 μg/mL. The method yields results comparable to those of the calorimetric method using Coomassie Brilliant Blue G-250 (CBB) with relative standard deviations of 0.72–2.10% (n = 10). There is almost no interference by amino acids and most of the metal ions.     

Aggregation and photobleaching of merocyanine 540 as probed by resonance light scattering

Merocyanine 540 (MC540) aggregation induced by adding KCl has been studied by resonance light scattering (RLS) and absorption spectrophotometry. In water, MC540 exists as H-dimers and monomers with absorption maxima at ～500 and 535 nm, respectively (these species lack RLS). Upon the introduction of the salt in concentrations below 0.15 M, the spectrum undergoes a hypochromic effect, without modification of its general shape. In addition to the hypochromic effect, a new broad RLS band emerges at ～420–460 nm, which arises from large H-aggregates of the dye. The formation of these aggregates does not manifest itself in absorption spectra. At KCl concentrations above the critical one (0.15 M), a new absorption band at ～517 nm emerges; simultaneously, a strong RLS band of a similar shape appears, which proves the formation of large supramolecular aggregates of MC540. Comparison of the spectrophotometry and RLS data shows that large aggregates of MC540 are more photolabile than dimers and monomers.     

灿烂甲酚蓝共振光谱散射法测定脱氧核糖核酸

研究了灿烂甲酚蓝与脱氧核糖核酸（DNA）作用的共振光散射光谱,在pH＝10．8－11．5的范围内,DNA的加入导致灿烂甲酚蓝共振光散射的增强,在347nm处,存在一共振光散射增强峰,其强度与DNA的浓度呈线性关系,据此建立了一种测定DNA的共振光谱散射法。该方法的线范围为80－100μg/L,检出限为23．3μg/L.     

基于与铁氰化钾和Zn~(2+)作用共振光散射法测定异烟肼

在酸性介质中,异烟肼能将铁氰酸根离子还原成亚铁氰酸根离子,后者与硫酸锌反应生成K2Zn3[Fe(CN)6]2粒子引起体系的共振光散射信号显著增强.在345nm处增强的散射信号强度ΔIRLS与异烟肼的浓度在0.01~1.0μg/mL范围内呈线性关系,据此建立了一种检测异烟肼含量的共振光散射(RLS)分析方法.线性回归方程为ΔIRLS=136.1+4239c(c,μg/mL),相关系数(r)为0.9984,检测限(3σ)为3.8ng/mL.该方法已成功用于异烟肼片剂及血清样品的测定.此外,文中还结合吸收光谱,动态光散射,扫描电子显微镜等表征手段对反应机理和RLS信号强度增强的原因进行了探讨.     

Resonance light scattering properties of Eu3+ in gold colloid

Gold colloidal containing rare-earth ions Eu3+ were prepared at room temperature. Fluorescence spectra and resonance light scattering (RLS) spectra of Eu3+ ions and gold colloid containing Eu3+ were measured. For solution containing Eu3+, RLS features show two peaks at the edges of the visible light wavelength region. The short wavelength peak takes place at about 400 nm and the longer wavelength peak is the corresponding 1/2 fraction frequency RLS peak, which takes place at about 780 nm. When gold colloids were added to the solution containing Eu3+, both these two RLS peaks were enhanced. We believe that the energies, which are absorbed by the surface plasmon resonance in the gold nanoparticles, are efficiently transferred into the Eu3+ ions to cause the increased scattering.     

Determination of trace metallothioneins at nanogram levels with Eosin Y by resonance light scattering method

The interactions of metallothioneins with Eosin Y were studied by the absorption spectra and resonance light scattering (RLS) spectra methods. A direct RLS spectra method was applied for the determination of trace metallothioneins. The interaction of Eosin Y and metallothioneins enhanced the RLS intensity of system in Britton-Robinson buffer (pH 3.91), with the help of anionic surfactant (sodium dodecyl benzene sulphate). The mechanism was studied and discussed in terms of the RLS and UV-absorption spectra. Under optimal experimental conditions, at 366 nm, there was a linear relationship between the RLS intensity and the concentration of the metallothioneins in the range of 0.04–14.0 μg mL^?1, with a correlation coefficient of r = 0.9985 and detection limit of 11.9 ng mL^?1. The relative standard deviation was 3.1% (n = 11), and the average recovery was 95.2%. The method proposed was reliable, selective and sensitive in determining trace metallothioneins in human urine samples with the results in good agreement with those obtained by high-performance liquid chromatography.     

中性介质中中性红与双链DNA作用的光谱

通过分子吸收、荧光发射和共振光散射测定,表征了在水溶液介质中中性红(NR)与双 螺旋DNA的作用.在pH 7.63和离子强度低于0.01的水溶液介质中,随着NR与DNA的摩尔比(R)变 化,存在有两种结合方式.第一种结合方式发生在R > 2.22,此时获得共振光散射光谱增强信 号,表明NR在DNA分子表面发生聚集,集聚特性可使用RLS测定数据进行Scatchard分析;第二种 结合方式发生在R < 2.22,此时NR内嵌到DNA分子的双链碱基对之间,具有特征波长红移和分 子吸收增色效应,发生了从DNA到NR的分子能量转移,能观察到荧光增强.     

A sensitive resveratrol assay with a simple probe methylene blue by resonance light scattering technique

A novel resonance light scattering (RLS) method was developed for the determination of resveratrol based on the interaction between resveratrol and methylene blue (MB). It was found that at pH 8.69, the weak RLS intensity of MB was remarkably enhanced by the addition of trace amount of resveratrol with the maximum peak located at 385.0 nm. Under the optimum conditions, a good linear relationship between the enhanced RLS intensities and the concentrations of resveratrol was obtained over the range of 2.0-14.0 μg ml(-1) with the detection limit (3σ) of 0.63 μg ml(-1). The results of the analysis of resveratrol in synthetic samples and human urine are satisfactory, which showed it may provide a more sensitive, convenient, rapid and reproducible method for the detection of resveratrol, especially in biological and pharmaceutical field. In this work, the characteristics of RLS, absorption and fluorescence spectra of the resveratrol-MB system, the influencing factors and the optimum conditions of the reaction were investigated.     

J-aggregates of diprotonated tetrakis(4-sulfonatophenyl)porphyrin induced by ionic liquid 1-butyl-3-methylimidazolium tetrafluoroborate

The J-aggregation behavior of diprotonated tetrakis(4-sulfonatophenyl)porphyrin (H2TPPS4(2-)) in aqueous solution in the presence of the hydrophilic ionic liquid 1-butyl-3-methylimidazolium tetrafluoroborate (bmimBF4) was investigated in detail using UV-vis absorption spectroscopy, fluorescence spectroscopy, resonance light scattering (RLS) spectroscopy, Raman spectroscopy, and nuclear magnetic resonance (NMR) spectroscopy. With the addition of bmimBF4, increasing peaks appeared at a wavelength of 490 nm in the absorption spectra to account for the formation of H 2TPPS4(2-) J-aggregates. In addition, the experimental results also showed decreased fluorescence emission, enhanced RLS signals, intensified Raman scattering peaks, and the disappearance of NMR signals to further indicate that porphyrin J-aggregates exist in the studied system. NMR shifts of bmimBF 4 toward high field occurred corresponding to H2, H4, and H5 in the cationic imidazolium ring (bmim+), suggesting that bmim+ enters the magnetic shielding domain of the anionic phenyl sulfonate ion owing to the association process between the "large" cation and anion. Additionally, the fact that the absorption spectral shifts occurred in the nonprotonated porphyrin TPPS4(4-) further indicates the existence of the ion association effect of bmim+, which functions as an important factor in porphyrin aggregation.