共振散射光谱法研究人血清白蛋白与二甲酚橙的反应

对二甲酚橙作为光散射探针测定蛋白质进行了研究,基于人血清白蛋白对二甲酚橙的共振光散射强度的增强效应,建立了测定蛋白质的共振散射光谱法。在pH 4.00的NaOAc-HOAc缓冲溶液中,二甲酚橙只有微弱的光散射强度,但它与蛋白质的缔合物却有较强的共振光散射信号,在λ=517 nm处,光散射强度达到最大,并且与蛋白质浓度在为0.0~10.0 mg.L-1范围呈线性,检出限为0.044 mg.L-1。运用摩尔比法测定二甲酚橙和蛋白质的结合数为132,用于实际样品的分析,测定值与考马斯亮蓝法的结果一致,分析结果的RSD值(n=5)均小于5%。     

藉L-半胱氨酸包覆的ZnS纳米粒子的共振光散射定量分析蛋白质

合成和表征了功能性L-半胱氨酸包覆的ZnS纳米粒子。在pH5．12的NaAc-HAc溶液介质中,L-半胱氨酸包覆ZnS纳米粒子于波长308．0nm处出现共振光散射峰。一定量蛋白质的加入能明显增强体系的共振光散射,且峰强度增加值与蛋白质浓度间存在良好线性关系,据此建立了一种灵敏的测定微量蛋白质的方法。用L-半胱氨酸包覆ZnS纳米粒子作为探针,不仅克服了有机染料可能出现的光漂白等缺点,而且本身不具毒性。该法用于人血清试样中总蛋白的测定,其结果与临床数据一致。     

溴酚蓝共振光散射探针测定敦煌壁画胶结材料中蛋白质含量

溴酚蓝共振光散射探针测定敦煌壁画胶结材料中蛋白质含量;敦煌壁画; 颜料胶结剂; 共振光散射; 蛋白质; 溴酚蓝     

三种偶氮化合物的荧光光谱研究

近年来 ,一些重要的有机染料探针在生物大分子光度分析、荧光分析和共振光散射分析方面得到了日益广泛地应用[1,2 ] ,深入研究这些有机染料的结构和光谱特性 ,探讨这些有机染料与生物大分子之间的作用 ,对于筛选性能优良的分子光谱探针 ,设计更加灵敏简便的分子光谱检测器件 ,是现代分析化学十分重要的课题。本文测定了偶氮胂Ⅱ (Ａｒｓｅｎａｚｏ)、铬黑Ｔ(ＥｒｉｏｃｈｒｏｍｅｂｌａｃｋＴ)、铬蓝黑 (ＥｒｉｏｃｈｒｏｍｅｂｌｕｅｂｌａｃｋＲ)等 3种化合物的荧光光谱 ,并用量子化学半经验方法ＡＭ1和ＰＭ3对3种化合物分子进行包括构型…     

共振光散射探针铁的混配物的合成及其在脱氧核糖核酸测定中的应用

1　引　　言共振光散射技术在测定核酸方面有较广阔的应用前景。而在核酸探针的探索中 ,人们发现邻菲咯啉、联吡啶等大环配体有共轭π键和刚性平面 ,可进行手性异构体的识别。本实验合成了铁 与邻菲咯啉、联吡啶的混配物 ,并通过紫外、荧光和共振光散射等技术研究了混配物与DNA作用状况 ,证明此混配物可作为脱氧核糖核酸的共振光散射探针 ,且定量测定DNA时灵敏度高。2　实验部分2 .1　仪器与试剂　GSP 77 0 3磁力搅拌器 (江苏秦县医疗器械厂 ) ;RF 5 40荧光分光光度计 (日本岛津公司 ) ;λ 17型紫外 可见分光光度计 (美国P E公司 ) …     

具有核酸分子"光开关"特性钌(Ⅱ)配合物的研究进展

钌（Ⅱ）配合物类核酸分子“光开关”探针性质稳定、无毒环保,可用于痕量核酸检测、基因序列分析及三链DNA检测、DNA图像研究及DNA动力学过程分析、基因损伤研究、基因转染材料研究、量子点生物效应研究及用作电化学探针。随着核酸及其相关分析研究的不断深入和适配子技术的迅猛发展,基于核酸和核酸分子“光开关”还可进行药物筛选、生命活性分子如ATP及蛋白质等的分析检测,具有简便、快速、灵敏、抗光漂白等特性。对生命科学基础研究、食品安全及医学诊断具有重要的理论意义。作者对近10年来核酸分子“光开关”探针研究进展进行了评述,引用文献55篇。     

用铬黑T作为共振光散射探针测定蛋白质

研究了金属指示剂铬黑T（EBT）作为共振光散射探针测定蛋白质的分析方法。实验表明，在pH=4.10的Britton-Robinson缓冲溶液条件下，铬黑T只有极弱的光散射，它与蛋白质结合后有强烈的共振光散射作用。在λ=375nm处，光散射强度最大，光散射强度与蛋白质的浓度成正比。据此建立了一种测定蛋白质的新方法。该方法简便、快速、灵敏度高，对HSA的检出限达到39μg/L;线性范围为0－15mg/L，用于人体血清样品的分析并用考马斯亮蓝法比较，取得了令人满意的结果。同时亦研究了牛血清白蛋白（BSA）、λ球蛋白、鸡蛋白蛋白、溶菌酶与染料EBT之间的作用。比较了2种不同类型的荧光仪器绘制的共振光散射光谱，并探讨了共振光散射的机理。     

亮黄-曲通X-100体系共振瑞利散射法测定蛋白质

基于在TrtionX-100存在下，蛋白质对有机染料亮黄瑞利光散射的增强作用。拟定了测定蛋白质的瑞利光散射光，由于添加了TritonX-100，对不同的蛋白质，测定的灵敏度提高了5－11．8倍，线性范围在0－5．0mg/L之间，最低检测限为10．2μg/L。     

功能性CdS纳米荧光探针荧光增敏法测定人血清白蛋白

目前 ,以荧光分析法对蛋白质进行研究主要采用有机荧光探针[1～ 3 ] .与传统的有机染料 (如罗丹明 )探针相比 ,半导体纳米晶体探针的光强度要高 2 0倍 ,光稳定性要高 1 0 0倍 ,谱线宽度只是有机染料谱线宽度的 1 /3 [4 ] .将半导体纳米晶体作为探针用于测定生物分子 ,将大大提高分析的灵敏度和选择性 ,而目前其应用于生物染色、医疗诊断、DNA序列测定和免疫分析等方面的研究很少 [4 ,5] .本文合成了胶态纳米粒子 Cd S,并在其外表面修饰一层巯基乙酸 ,使其具有水溶性 ,并能与生物分子作用 ,从而可利用其外表面的功能性基团对人血清白蛋白进…     

聚二烯丙基二甲基氯化铵与核酸相互作用的共振光散射光谱及分析应用

实验基于核酸与聚阳离子聚二烯丙基二甲基氯化铵(PDDA)的相互作用导致共振光散射(RLS)增强的现象来测定核酸。考察了pH值、PDDA浓度和离子强度对体系共振光散射强度的影响。在优化条件下,建立了用RLS光谱测定微量核酸的新方法。方法的抗干扰能力较强,可允许大部分的常见金属离子、核苷酸、氨基酸、糖、蛋白质等干扰物质的存在。同时用于合成样品的分析,结果令人满意。     

有机染料共振光散射法测定蛋白质的研究进展

对用有机染料作试剂的共振光散射光谱法测定蛋白质研究的进展情况(主要包括1990年至2004年间)作了评述。对测定蛋白质的反应体系中有机染料作用的基本原理作了简要论述。文中涉及的有机染料主要有:三苯甲烷类、偶氮类、酞菁类及羟基蒽醌类等(引用文献58篇)。     

A High-Sensitivity Assay of Nucleic Acids with Tetraphenyl Porphyrin Cobalt Chlorine by Resonance Light Scattering Technique

Abstract

A novel probe, tetraphenyl porphyrin cobalt chlorine (CoTPPCl), is first applied to determine nucleic acids at the nanogram level based on the measurement of resonance light scattering (RLS) signals, which result from the interaction of CoTPPCl with nucleic acids. Under pH 6.37 conditions, the reaction between CoTPPCl and nucleic acid enhances the weak resonance light scattering (RLS) signal of CoTPPCl, and the enhanced light scattering intensity is proportional to the concentration of nucleic acid. The method is sensitive (3.45 ng/mL for ctDNA), simple (one step and a common fluorimeter), and tolerant of the metal ions and other coexistent substances. The mode of the combination between CoTPPCl and nucleic acids and the reasons for RLS enhancement are clearly clarified. Synthetic samples were determined with satisfactory results.     

Determination of nucleic acids in acidic medium by enhanced light scattering of large particles

The large particle light scattering technique was first developed as a sensitive and convenient analysis method for microdetermination of nucleic acids by using a common spectrofluorometer. In 0.1 mol l(-1) HCl, H(2)SO(4), or HNO(3) solution, the nucleic acids can aggregate to form large particles whose dimensions are comparable to the wavelength of UV-Vis light. The large particles can result in very strong light scattering which is well proportional to the concentration of nucleic acids in the range of 0.06-100.0 mug ml(-1) for calf thymus DNA, 0.05-60.0 mug ml(-1) for fish sperm DNA, and 0.6-90.0 mug ml(-1) for yeast RNA. The detection limits (3sigma) are 18.0 ng ml(-1) for calf thymus DNA, 16.0 ng ml(-1) for fish sperm DNA, and 57.6 ng ml(-1) for yeast RNA, respectively. Six synthetic samples were determined with satisfactory results.     

Mapping of surrogate markers of cellular components and structures using laser desorption/ionization mass spectrometry

Laser desorption/ionization mass spectrometry (LDI-MS) has been used to assess the potential of using surrogate markers, bound to cellular structures containing nucleic acids, to image or map the position of these structures within biological samples. In this study, organic dyes were used as markers because of their established use in the histochemical marking of nucleic acids, and also because they are amenable to LDI-MS. Eight cationic dyes were tested and all could be desorbed from nucleic acid samples without additional matrix after specifically binding to these molecules. Methylene Blue was the best of these based on its sensitivity to detection by LDI-MS and the fact that it can be washed from the tissue in areas where it was not specifically bound to provide low-intensity background signals. Experiments are reported which characterize the M(+) ion signal obtained from Methylene Blue with regard to sensitivity, reproducibility and possible use for quantitation. This dye was used to map (with a lateral resolution of 25 microm) several nucleic acid-containing samples spotted on prepared surfaces, and to image the location of nucleic acids in two model tissues, retinal vertical sections and thyroid whole mount sections.     

Properties of nucleic acid staining dyes used in gel electrophoresis

Nucleic acid staining dyes are used for detecting nucleic acids in electrophoresis gels. Historically, the most common dye used for gel staining is ethidium bromide, however due to its toxicity and mutagenicity other dyes that are safer to the user and the environment are preferred. This Short Communication details the properties of dyes now available and their sensitivity for detection of DNA and their ability to permeate the cell membrane. It was found that GelRed? was the most sensitive and safest dye to use with UV light excitation, and both GelGreen? and Diamond? Nucleic Acid Dye were sensitive and the safer dyes using blue light excitation.     

Interactions of Night Blue with Nucleic Acids and Determination of Nucleic Acids Using Resonance Light Scattering Technique

The noncovalent interactions of night blue (NB) with several nucleic acids in buffer medium of Britton‐Robinson at pH 4.1 have been studied by spectroscopic methods. It is shown that the binding of NB with nucleic acids involves the J‐aggregation of NB molecules on the surface of nucleic acids. The aggregation was encouraged by polyanions nucleic acids, in which nucleic acids served for acting templates. In this connection, a new method of nucleic acids with sensitivity at nanogram level is proposed based on the measurement of enhanced resonance light scattering (RLS). The linear range of ctDNA, fsDNA and yRNA is 0.01—2.5, 0.03—2.5 and 0.04—1.0 μg/mL, respectively, and the corresponding detection limits (3s?) are 9.4, 7.3 and 5.7 ng/mL at 2.5 × 10–⁵mol/L of NB. Synthetic and real samples were analyzed with satisfactory results.     

Nephelometric determination of micro amounts of nucleic acids with protamine sulfate

Nucleic acids can form large particle complexes with protamine sulfate by electrostatic forces, which results in strong light scattering. Based on this, a nephelometric method is described for sensitive and convenient determination of nucleic acids with protamine sulfate by using a common spectrofluorimeter. Maximum light scattering is produced in the range of pH 2.2-4.4 with the same excitation and emission wavelengths at 365 nm. Under optimal conditions, the calibration curves are linear in the range 0.05-60.0 micrograms cm-3 for nucleic acids. The corresponding detection limits are 12.5 ng cm-3 for calf thymus DNA, 9.0 ng cm-3 for fish sperm DNA, and 18.0 ng cm-3 for yeast RNA, respectively. Six synthetic samples are determined with satisfactory results. The relative standard deviation of five replicate measurements is 3.2% for 2.0 micrograms cm-3 calf thymus DNA.     

Key Structural Elements of Unsymmetrical Cyanine Dyes for Highly Sensitive Fluorescence Turn‐On DNA Probes

Unsymmetrical cyanine dyes, such as thiazole orange, are useful for the detection of nucleic acids with fluorescence because they dramatically enhance the fluorescence upon binding to nucleic acids. Herein, we synthesized a series of unsymmetrical cyanine dyes and evaluated their fluorescence properties. A systematic structure–property relationship study has revealed that the dialkylamino group at the 2‐position of quinoline in a series of unsymmetrical cyanine dyes plays a critical role in the fluorescence enhancement. Four newly designed unsymmetrical cyanine dyes showed negligible intrinsic fluorescence in the free state and strong fluorescence upon binding to double‐stranded DNA (dsDNA) with a quantum yield of 0.53 to 0.90, which is 2 to 3 times higher than previous unsymmetrical cyanine dyes. A detailed analysis of the fluorescence lifetime revealed that the dialkylamino group at the 2‐position of quinoline suppressed nonradiative decay in favor of increased fluorescence quantum yield. Moreover, these newly developed dyes were able to stain the nucleus specifically in fixed HeLa cells examined by using a confocal laser‐scanning microscope.     

Interaction of Crown Ether‐Annelated Styryl Dyes with Double‐Stranded DNA

DNA‐binding properties of 15‐crown‐5‐derived mono‐ and bis‐styryl dyes were investigated in the presence of calf thymus DNA. To access the factors that influence the DNA association in the series of these ligands, the structure of the molecules was varied by either changing size of the heterocyclic moiety or altering the position of the styryl substituents. The major binding mode for the monostyryl dyes is intercalation. Notably, binding of the dyes to the nucleic acids leads to a fluorescence enhancement by a factor of up to 54. Therefore, these cationic styryl derivatives may be applied as fluorescent “light‐up” probes for DNA detection.