铬天青S共振光散射法测定脱氧核糖核酸

介绍在阳离子表面活性剂十六烷基三甲基溴化铵(CTMAB)存在下阴离子染料铬天青S(CAS)共振光散射(RLS)法测定脱氧核糖核酸(DNA)的方法。在pH=5．27的六次甲基四铵一盐酸缓冲溶液中，研究了CAS—CT-MAB—yDNA体系的RLS光谱特征、影响因素和最佳反应条件。在最佳条件下，体系的RLS强度增加值△I与yDNA的浓度在50～800μg／L和1000～2000μg／L呈线性关系，其线性回归方程分别为△I=0．48c 2．56和△I=0．14c 17．86，相关系数分别为0．9997和0．9991，检出限为4．3ng／mL。该方法简便、快速，应用于合成样品中yDNA的测定，测定结果的相对标准偏差为2．93％～4．71％，回收率为97．8％～105．2％。     

铝离子与脱氧核糖核酸作用的共振光散射研究

在PH2．21的酸性介质中，Al^3 与脱氧核糖核酸（DNA）发生静电作用产生以291．0nm为特征峰的共振光散射（RLS）增强光谱，即Al^3 主要与DNA分子表面的磷酸根结合，但DNA热变性将导致Al^3 与DNA的碱基结合，使光散射信号降低，在291．0nm处的共振光散射（RLS）强度与DNA的浓度呈线性关系，据此建立了用共振光散射测量痕量DNA的新方法，方法的检出限为ng级，用于合成样分析，回收率在91．6％－105．0％。     

荧光素共振光散射法测定脱氧核糖核酸

研究了咕吨类染料荧光素Fluorescein(FL)与DNA作用的共振光散射光谱。加入DNA后,在pH6～8的范围内,荧光素在DNA分子表面发生长距离自组装,在400nm处产生了增强的共振光散射峰,其发光强度与DNA的浓度呈线性关系,线性范围为0．04～3．1mg／L;检出限为16μg／L。考察了影响因素和最佳反应条件,建立了用RLS光谱测定ng级DNA的新方法。     

流动注射-共振光散射联用技术测定注射液中肝素的含量

在近中性介质中,亚甲基兰与肝素作用产生共振光散射（BLS）增强信号,最大散射峰位于365．0nm处,增强的共振光散射强度（DIRLS）与肝素浓度具有线性关系,据此建立了流动注射．共振光散射联用技术测定痕量肝素的新方法。在pH为7．96,离子强度为0．0275mol／L的载流中加入肝素后,在365．0nm处产生增强的RLS信号。采用时间扫描测定该增强RLS强度,在最佳实验条件下,可检测1～20mg／L肝素,检出限为8．41mg／L。对浓度为4．0mg／L的肝素钠标准液平行测定11次的相对标准偏差为3．2％。用于注射液中肝素含量的测定,RsD小于2．3％。     

吖啶橙共振光散射法测定痕量脱氧核糖核酸

研究了三环杂芳香类染料吖啶橙(AO)与DNA作用的共振光散射光谱,在pH11．5～12．5的范围内,加入DNA导致吖啶橙共振光散射增强,在339nm处,存在一共振光散射增强峰,其强度与DNA浓度呈线性关系,据此建立了一种测定DNA的共振光散射新方法?对于ctDNA,方法的线性范围为14．3～1000μg／L,检出限为2．86μg／L,RSD为3．6％;对于fsDNA,方法的线性范围为24．0～1250μg／L,检出限为4．78μg／L,RSD为6．0％。已用于合成样品中DNA的测定。     

罗丹明6G与核酸作用的共振光散射光谱及其分析应用

研究了罗丹明6G（Rh6G）与核酸（ctDNA和yRNA)作用的共振光散光谱（RLS）特征，基于RLS的增强，建立了一种测定核酸的新方法，考察了各种影响因素，在优化条件下确定了RLS强度与ctDNA和yRNA浓度之间的关系，相应的线性范围分别为0.05-37.0μg.mL^-1、0．1－10．0μg.mL^-1，检出限分别为3．0ng.mL^-1和9．5ng.mL^-1。四种合成样品五次平行测定结果的相对标准偏差（RSD）范围为2．0％－3．0％。     

钨酸钠-罗丹明B-P体系共振光散射法对甲拌磷残留的测定

研究了共振散射技术测定甲拌磷残留的新方法。实验结果表明,酸性溶液中,甲拌磷和钨酸钠相互作用能够形成杂多酸,该杂多酸与碱性三苯甲烷染料罗丹明B（RhB）结合,形成了缔合物粒子,导致体系在λex/λem=606nm共振散射（RLS）强度急剧增强,并产生新的RLS光谱。在选定的实验条件下,甲拌磷浓度在0．43-200nmol／L范围内,与体系的RLS强度有良好的线性关系（r=0．9977）,据此建立了共振散射法快速测定甲拌磷的新方法,该法检出限为0．057nmol／L,回收率为82％～99％,用于蔬菜样品中甲拌磷残留量的测定,与气相色谱法对照,结果满意。     

耐尔蓝硫酸盐在核酸分子表面的长距组装及核酸的三波长共振光散射测定

在pH7.20～7.60及离子强度低于0.012的介质中,耐尔蓝硫酸盐(NBS)在核酸分子表面进行长距组装后,产生293.4nm、349.4nm和560.4nm的共振光散射(RLS)增强峰.根据RLS增强的Scatchard数据分析表明,NBS在小牛胸腺DNA、鱼精DNA和酵母RNA上的组装数分别是6.4、6.6和3.9,组装常数分别为7.1×10~6mol/L、4.6×10~6mol/L和1.7×10~6mol/L.应用三个波长处的RLS增强之和可以测定0～0.8mg/L的小牛胸腺DNA、鱼精DNA和0.20～0.60mg/L的酵母RNA,检测限分别是0.4、1.2和10.5μg/L.方法已成功的应用于合成样测定.     

CTMAB与DNA相互作用的共振光散射研究及其应用

应用共振光散射(resonance light scattering,RLS)光谱法对十六烷基三甲基溴化胺(CTMAB)与小牛胸腺DNA(ct DNA)相互作用进行了研究,并研究了该体系的最佳反应条件.发现CTMAB可提高ct DNA的RLS信号.采用该方法对合成样品进行了分析测定,回收率和RSD分别为94.8%~97.3%和1.1%~2.5%,检出限为9.3μg/L.     

紫外灯照射牛血清白蛋白的共振光散射光谱法测定

利用紫外灯照射后牛血清白蛋白(BSA)的共振光散射(RLS)强度的增强,建立了一种快速、简便测定BSA的RLS光谱法。考察了pH值、反应最佳时间等因素对RLS强度的影响。实验结果表明,在pH值为4.95,紫外灯照射时间为90min条件下,测定BSA的线性范围为0.5～10mg/L,检出限为0.33mg/L。同时发现DNA与BSA共同作用时,RLS强度增强幅度增加,测定BSA的线性范围为0.05～10mg/L,检出限为0.01mg/L。将该法应用于合成样品中BSA测定,结果较好。     

核酸对氯化银胶体溶液共振光散射的猝灭作用及其应用

报道了一种测定水溶液中核酸的方法,该法基于核酸对氯化银溶胶共振射光的猝灭作用。在理想测定条件下,散射光的猝灭程度正比于核酸的浓度,三种核酸（ｃａｌｆ ｔｈｙｍｕｓ ＤＮＡ,ｈｅｒｒｉｎｇ ＤＮＡ ａｎｄ ＹｅａｓｔＲＮＡ）的线性范围分别为０－２０μｇ／Ｌ,０－６０μｇ／Ｌ和０－８０μｇ／Ｌ,检测限分别为０．６５μｇ／Ｌ,１．１μｇ／Ｌ和１．９μｇ／Ｌ。６种合成样品的测定结果令人满意,机理研究结果表明,核酸中的碱基（尤其是嘌呤碱）同银离子具有很强的结合能力,这种结合影响了氯化银的沉淀平衡,导致了氯化银溶胶共振散射光的猝灭。     

十六烷基溴化吡啶与脱氧核糖核酸作用的共振光散射光谱及其分析应用

在碱性条件下，十六烷基溴化吡啶(CPB)与脱氧核糖核酸(DNA)共存时，体系产生较强的共振光散射，其强度与DNA浓度呈线性关系，据此提出了基于阳离子表面活性剂的共振光散射法定量测定DNA。在最佳实验条件下，测得小牛胸腺DNA(ctDNA)和鱼精子DNA(fsDNA)的线性范围分别为0．2-2．0mg／L和0．2—1．25mg／L，检出限分别为0．07mg／L和0．05mg／L。该方法已应用于合成样品及实际样品中DNA含量的测定。     

花菁-脱氧核糖核酸的共振光散射光谱及其分析应用

研究了一种苯并噻唑阳离子花菁与脱氧核糖核酸(DNA)作用的共振光散射光谱,在pH 6.0的六次甲基四胺-HCl缓冲介质中,痕量DNA的加入使花菁在590nm的共振光散射强度显著增强。在最佳实验条件下,增强的共振光散射强度与DNA浓度具有良好的线性关系,据此建立了一种测定DNA的共振光散射光谱法。方法的线性范围为:小牛胸腺DNA(CT DNA),0～20μg/mL,鱼精子DNA(FS DNA),0～15μg/mL;检出限分别为0.005μg/mL和0.008μg/mL。该方法已用于合成样品中DNA的测定。     

Multi-spectroscopic method study the interaction of anti-inflammatory drug ketoprofen and calf thymus DNA and its analytical application

Interactions of the anti-inflammatory drug ketoprofen with calf thymus DNA (ctDNA) in aqueous solution have been studied by multi-spectroscopic method including resonance light scattering (RLS) technique, ultraviolet spectra (UV), (1)H NMR, etc. The characteristics of RLS spectra, the effective factors and optimum conditions of the reaction have been unequivocally investigated. Mechanism investigations have shown that ketoprofen can bind to ctDNA by groove binding and form large particles, which resulted in the enhancement of RLS intensity. In Critic acid-Na(2)HPO(4) buffer (pH=6.5), ketoprofen has a maximum peak 451.5 nm and the RLS intensity is remarkably enhanced by trace amount of ctDNA due to the interaction between ketoprofen and ctDNA. The enhancement of RLS signal is directly proportional to the concentration of ctDNA in the range of 1.20×10(-6)-1.0×10(-5) mol/L, and its detection limit (3σ) is 1.33×10(-9) mol/L. The method is simple, rapid, practical and relatively free from interference generated by coexisting substance, and was applied to the determination of trace amounts of nucleic acid in synthetic samples with satisfactory results.     

Determination of DNA with cetyltrimethylammonium bromide by the measurement of Resonance Light Scattering.

A simple assay of DNA was developed based on the measurements of enhanced signals of Resonance Light Scattering (RLS) of cetyltrimethylammonium bromide (CTMAB) by DNA. The enhanced RLS signals, measured by simultaneously scanning the excitation and emission monochromators of a common spectrofluorometer with lambda ex = lambda em, was optimized for the DNA assay with CTMAB. On the conditions of pH 2.21 and ionic strength 0.002, the enhanced RLS intensity at 470.0 nm, delta I, was found to be proportional to the concentration of DNA in the range 0-2.5 micrograms/ml if 1.5 x 10(-5) M CTMAB was used. Limits of determination for calf thymus DNA and fish sperm DNA were 4.9 ng/ml and 9.2 ng/ml, respectively. Synthetic samples were determined with the recovery ratio ranging from 93.2% to 105.1%, and the RSD is lower than 2.7%.     

Determination of serum albumin in the presence of poly(diallyldimethylammonium chloride) by resonance light scattering technique

By means of the resonance light scattering (RLS) technique, a new method was developed to determine the bovine serum albumin (BSA) and human serum albumin (HSA) by the interaction of serum albumin with poly(diallyldimethylammonium chloride) (PDDA). At Tris-NaOH buffer solution, the RLS intensity of serum albumin at the wavelength 320, 550 and 590 nm was obviously enhanced in the presence of PDDA. The influences of some experimental factors, including incubation time, addition sequence of reagents, pH value, concentration of PDDA and foreign substances, on the enhancement of the RLS intensity were examined. The optimum conditions of the experiment were selected. Under the selected experimental condition, the enhanced RLS intensities were directly proportional to the concentrations in the range of (0.0250-2.75)x10(-6) mol/L for BSA and (0.0235-1.17)x10(-6) mol/L for HSA. The detection limits (S/N=3) were 8.40x10(-9) mol/L for BSA and 7.39x10(-9) mol/L for HSA. The synthetic samples were analysed and the results obtained were satisfactory.     

DNA对Ru(bpy)_2(dppx)~(2+)-SDS体系共振光散射的猝灭作用及其应用

研究了Ru(bpy)2(dppx)2+-SDS-DNA(bpy=2,2′-联吡啶,dppx=7,8-二甲基-吡啶并[3,2-a:2′,3′-c]吩嗪)体系的共振光散射光谱。结果表明,在阴离子表面活性剂十二烷基硫酸钠(SDS)预胶束聚集体存在下,Ru(bpy)2(dppx)2+-SDS体系具有很强的共振光散射,DNA的加入使其共振散射光猝灭。探讨了反应机理。基于DNA对Ru(bpy)2(dppx)2+-SDS体系共振光散射的猝灭作用,建立了共振光散射法测定DNA的新方法。在最佳实验条件下,体系在393nm处的共振光散射猝灭程度与DNA的浓度呈线性关系,线性范围为0.01～1.2mg/L,检出限为1.5μg/L。     

Determination of a cationic surfactant with naphthalene black 12B by the resonance light scattering technique

A new determination method for a cationic surfactant, zephiramine (Zeph), was developed with resonance light scattering (RLS) technique, based on the interaction of naphthalene black 12B with Zeph. The resonance light scattering (RLS) and UV characteristics of interaction between naphthalene black 12B and Zeph were studied. The RLS intensity of naphthalene black 12B at 363 nm was greatly enhanced in the presence of Zeph at pH 6.0. The enhanced RLS is proportional to the concentration of Zeph in the range of 3.20 x 10(-7) - 1.44 x 10(-5) mol L(-1). The limit of detection was 8.8 x 10(-8) mol L(-1). The proposed method was applied to the determination of Zeph in synthetic and spiked water samples with the recovery of 96.2-104% and RSD of 1.1-2.5%.     

Determination of deoxyribonucleic acids by a resonance light scattering technique and its application

For the first time, acetamiprid has been used to determine nucleic acid (DNA) using the resonance light scattering (RLS). The RLS of acetamiprid was greatly enhanced by DNA in the range of pH 1.6-1.8. A RLS peak at 313 nm was found, and the enhanced intensity of RLS at this wavelength was proportional to the concentration of DNA. The linear range of the calibration curve was 0-11.0 microg ml(-1) with the detection limit of 20 ng ml(-1). The nucleic acids in synthetic sample and in rice seedling extraction were determined satisfactorily. The interaction mechanism of acetamiprid and DNA is discussed. Mechanism studies show that the enhanced RLS is due to the aggregation of acetamiprid in the presence of DNA.     

Determination of bovine serum albumin using resonance light scattering technique with sodium dodecylbenzene sulphonate-cetyltrimethylammonium bromide probe

In this paper, the anionic surfactant sodium dodecylbenzene sulphonate (SDBS) and cationic surfactant cetyltrimethylammonium bromide (CTMAB) were used as resonance light scattering (RLS) probe to determine bovine serum albumin (BSA). Based on the weak RLS intensity of SDBS-CTMAB probe and the enhancement of RLS intensity of BSA in the presence of the probe, a simple assay for BSA was developed. The experimental results showed that the formation of three component complex BSA-SDBS-CTMAB is the main reason for the enhancement of RLS intensity of BSA, in which SDBS as a bridge can interact with both BSA and CTMAB. The effects of pH value, incubation time, concentrations of SDBS and CTMAB on the enhanced RLS intensity of BSA were investigated. Under the optimum conditions, the enhanced RLS intensity is proportional to the concentration of BSA in the range from 2.5 x 10(-8) to 2.0 x 10(-6)mol L(-1). The detection limit is 9.7 x 10(-9) mol L(-1) for BSA. The study of foreign substance effect on the determination of BSA indicated that most of metal ions have little effect on the determination of BSA. The results of assay for BSA in synthetic samples were satisfactory.