浊点萃取富集-石墨炉原子吸收光谱法同时测定环境水样和中药中超痕量铅和镉

提出了石墨炉原子吸收光谱法同时测定环境水样和中药中超痕量铅与镉的方法.以双硫腙为络合剂,在pH 7.0时,用Triton X-114非离子表面活性剂浊点萃取富集样品溶液中痕量铅和镉.用硝酸镁和磷酸二氢铵的混合液作为基体改进剂测定铅和镉,铅和镉的检出限(3s/k)分别为0.138,0.007μg·L-1,相对标准偏差(n=7)分别为1.90%,2.08%.对于10 mL样品溶液的富集倍数分别为18.3,17.7.应用所提出的方法测定了杨树叶(GBW 07604)和小麦粉(GBW08503)国家标准样品,测定结果与标准值相符.铅和镉的加标回收率分别为97.8%,94.0%(水样);98.0%,94.0%(中药样).     

浊点萃取-石墨炉原子吸收光谱法同时测定生物样品中痕量铅和镉

提出了石墨炉原子吸收光谱法同时测定小鼠肝中痕量Pb和Cd的方法。以8-羟基喹啉为络合剂,在pH 9.0时,用Triton X-100浊点萃取富集样品中的Pb和Cd。用NH4H2PO4作为基体改进剂测定Pb和Cd,Pb和Cd的检出限(3s/k)分别为0.103μg/L和0.0136μg/L,相对标准差(n=6)分别为1.4%,0.73%。对于10 mL样品溶液的富集倍数分别为7.1,9.3。利用该法分别测定了小鼠肝中的Pb和Cd的含量,加标回收率分别为96.4%～97.1%和101.3%～103.2%。     

浊点萃取-石墨炉原子吸收光谱法测定水样中痕量铝

提出了浊点萃取石墨炉原子吸收光谱法测定痕量铝的新方法。探讨了溶液pH、试剂浓度等实验条件对浊点萃取及测定灵敏度的影响。在最佳条件下,富集40 mL样品溶液,用石墨炉原子吸收光谱法测定,铝的检出限为0.045μg/L,铝的富集倍率为78.5倍。方法适用于自来水、河水及海水中痕量铝的测定。     

石墨炉原子吸收光谱法测定大白鼠脑组织中痕量铝

采用具有横向加热石墨炉原子化器系统和纵向塞曼效应背景校正的原子吸收光谱仪测定了大白鼠脑组织中痕量铝,并探讨了相关试验条件。采用全自动进样器进行标准在线稀释绘制工作曲线,同时进行在线添加基体改进剂和在线加标回收率试验。方法的特征质量为26.2 pg,检出限为11.6 pg,相对标准偏差为3.8%,回收率为91.6%~98.2%。     

浊点萃取-石墨炉原子吸收光谱法测定环境样品中的痕量镉

研究了浊点萃取-石墨炉原子吸收光谱法(GFAAS)测定痕量镉的新方法,利用表面活性剂Triton X-100和络合剂1-(2-吡啶偶氮)-2-萘酚(PAN)对镉进行浊点萃取。详细探讨了影响浊点萃取及测定灵敏度的因素。优化条件为:0.25 mL 30%NaC l,pH 8.5,0.50 mL、4.0×10-4mol/L PAN,0.2 mL 1.0%TritonX-100。在最佳条件下,镉的富集倍率为50倍,检出限为5.9 ng/L,RSD为2.1%。该方法用于环境样中痕量镉的富集和测定,结果令人满意。     

非螯合物浊点萃取-墨炉原子吸收法测定水中痕量铊（Ⅲ）

建立不需形成螯合物的浊点萃取-石墨炉原子吸收法测定水中铊a田D的新方法。用浊点萃取技术富集水中铊a田D，石墨炉原子吸收法测定。经考察，浊点萃取环境水体中铊a田D的最优条件为pH12，90℃水浴2h，Triton X-114浓度2．0g／L；在优化后实验条件下，方法测定铊a田D的检出限为0．018彬L；相对标准偏差为8．89％-13．7％（C=0．1μg／L及1．0μg／L，n：7）；加标回收率为98．0％-101％。本法适于水中痕量铊（Ⅲ）的测定。     

塞曼石墨炉原子吸收光谱法直接测定血液中痕量铝

采用偏振塞曼原子吸收法，以Ｃａ作基体改进剂，注入热解涂层石墨管中，直接测定用ＯＰ溶液稀释血液样品中的痕量铝，有效地消除了血液基体的干扰，克服了铝的记忆效应，从而提高了方法的测定灵敏度、重现性和准确度。     

石墨炉原子吸收分光光度法测定面制品中铝的含量

建立了石墨炉原子吸收光谱法测定面制品中铝含量的方法,经过一系列的条件实验及验证分析表明,方法标准曲线线性相关系数为0.999 2,相对标准偏差(RSD)为0.60%,加标回收率为98.3%~101%,方法灵敏度高,重现性好,结果准确可靠,能满足现有标准的检测要求。     

浊点萃取-火焰原子吸收光谱法测定水样中痕量铜的研究

提出了浊点萃取火焰原子吸收光谱法测定痕量铜的新方法。详细探讨了溶液pH，试剂浓度等实验条件对浊点萃取及测定灵敏度的影响，在最佳下，富集50mL样品溶液，用火焰原子吸收光谱法测定，铜的检测限为0.35μg/L，铜的富集倍率为71倍。方法用于自来水、河水及海水中痕量铜的测定。     

非螯合物浊点萃取-石墨炉原子吸收法测定水中痕量铊(Ⅲ)

建立不需形成螯合物的浊点萃取-石墨炉原子吸收法测定水中铊Ⅲ的新方法。用浊点萃取技术富集水中铊Ⅲ,石墨炉原子吸收法测定。经考察,浊点萃取环境水体中铊Ⅲ的最优条件为pH12,90℃水浴2h,Triton X-114浓度2.0g/L;在优化后实验条件下,方法测定铊Ⅲ的检出限为0.018μg/L;相对标准偏差为8.89%~13.7%(C=0.1μg/L及1.0μg/L,n=7);加标回收率为98.0%~101%。本法适于水中痕量铊Ⅲ的测定。     

Determination of human serum albumin using aurothiomalate as electroactive label

A new electroactive label has been used to monitor immunoassays in the determination of human serum albumin (HSA) using glassy-carbon electrodes as supports for the immunological reactions. The label was a gold(I) complex, sodium aurothiomalate, which was bound to rabbit IgG anti-human serum albumin (anti-HSA-Au). The HSA was adsorbed on the electrode surface and the immunological reaction with gold-labelled anti-HSA was then performed for one hour by non-competitive or competitive procedures. The gold(I) bound to the anti-HSA was electrodeposited in 0.1 mol L⁻¹ HCl at −1.00 V for 5 min then oxidised in 0.1 mol L⁻¹ H₂SO₄ solution at +1.40 V for 1 min. Silver electrodeposition at −0.14 V for 1 min followed by anodic stripping voltammetry were then performed in aqueous 1.0 mol L⁻¹ NH₃–2.0×10⁻⁴ mol L⁻¹ AgNO₃. For both non-competitive and competitive formats, calibration plots in the ranges 5.0×10⁻¹⁰ to 1.0×10⁻⁸ mol L⁻¹ and 1.0×10⁻¹⁰ to 1.0×10⁻⁹ mol L⁻¹ HSA, respectively, with estimated detection limits of 1.5×10⁻¹⁰ mol L⁻¹ (10 ng mL⁻¹) and 1.0×10⁻¹⁰ mol L⁻¹ (7 ng mL⁻¹), respectively, were obtained. Levels of HSA in two healthy volunteer urine samples were also evaluated, using both immunoassay formats.     

Determination of dissolved and particle-bound PCB congeners at ultra-trace concentrations in water

Adsorption of 10 PCB congeners in aqueous solutions on glass-fibre filters taken from different boxes but of the same type were not significantly different. The standard deviations using filters from the same box were below 10% at concentration levels of 4.1?ng?L^?1. At this level, the adsorption of dissolved PCB at the filters was in the range of 5–20% depending on the congener. This led to a procedure for determination of dissolved and particle-bound congener in authentic landfill leachate, which included correction for adsorption losses. The procedure was based on filtration through glass-fibre filters, followed by trapping of the PCB in the eluate on solid-phase extraction (SPE) disks. After separate supercritical fluid (SFE) extractions, with carbon dioxide, of the filters as well as of the SPE disks, the extracts were analysed on a two-column capillary GC-ECD system. Corrections for congener adsorption on glass-fibre filters were made, from which corrected distribution constants between particle-bound and dissolved PCB congener in the water phase could be obtained for authentic landfill leachate. These values (10⁴–10⁵) agreed well with those obtained by others.     

Interactions of bovine serum albumin with aluminum polyoxocations and aluminum hydroxide

Interactions of aqueous solutions of aluminum polyoxocations (Al13-mers and Al30-mers) and aluminum hydroxide suspensions of varying particle sizes (26, 55, and 82 nm) with a model protein, bovine serum albumin (BSA), have been investigated using potentiometry, conductometry, viscometry, 27Al solution NMR, UV-vis spectroscopy, dynamic light scattering, zeta-potential measurements, thermogravimetry, X-ray diffraction, and scanning electron microscopy. Increasing amounts of BSA partially convert Al13-mers and, to a larger extent, Al30-mers into amorphous Al hydroxide without gel formation. At the same time, BSA molecules can form unstable aggregates in the Al polyoxocation solutions which redisperse easily upon standing. In the case of Al hydroxide sols, BSA addition causes substantial gelation, the extent of which is proportional to the amount of BSA added and inversely related to the Al hydroxide particle size. Upon freeze-drying or centrifugation of Al species-BSA solutions, an interesting sheetlike morphology with 150-200 nm wide nanoribbons is observed for pure Al hydroxide nanoparticles and for solutions of Al polyoxocations with the highest amount of BSA studied. On the basis of the combined solution, colloidal and solid-state characterization of model Al species-BSA systems, a qualitative model of possible interactions in the Al polyoxocation-BSA and Al hydroxide-BSA systems is proposed wherein core-shell hybrid nanoparticles are formed from protein "core" and Al polyoxocation "shell" or Al hydroxide "core" and protein "shell".     

Determination of certain elements in human serum albumin by neutron activation analysis

Instrumental activation analysis was used to determine the contents of certain elements in human serum albumin (HSA). Sample irradiation was performed with a thermal neutron flux of 1.5·10¹³ n·cm⁻²·sec⁻¹ in the RA nuclear reactor of the Boris Kidrič Institute, Vinča. Measurements were performed on a 4096-channel analyser with a high-resolution Ge(Li) detector. The Na, Cu, Br, Au, Hg, Cr, Fe, Ag, Sc, Ba and Co contents were determined in HSA produced by the Institute for Blood Transfusion, Belgrade.     

TiO_2溶胶二级散射光谱法测定人血清白蛋白

制备了TiO2溶胶,并通过透射电子显微镜等对其结构进行了表征。研究了TiO2溶胶与人血清白蛋白(HSA)的相互作用。基于HSA对TiO2溶胶二级散射峰的增强作用,建立了二级散射光谱法测定痕量白蛋白的新方法。方法的线性范围是0.005~1.5 mg/L,检出限为3.5μg/L。方法用于人血中HSA的测定,回收率为98%~100.2%。     

In vitro detecting ultra-trace novalgin in medicine and human urine by chemiluminescence

A sensitive chemilumimetric method for the determination of novalgin at the sub-nanogram level is presented. The method is based on immobilized luminol and dichromate chemiluminescence detection coupled with a flow injection system. The intensity of the chemiluminescence can be strongly inhibited by novalgin and the decrement of CL intensity was linear with the logarithm of novalgin concentration in the range of 5.0×10⁻¹¹ to 5.0×10⁻⁸ g ml⁻¹. The detection limit is 2.0×10⁻¹¹ g ml⁻¹ (3σ) and the relative standard deviation is 2.57% (n=5) for a 1.0×10⁻¹⁰ g ml⁻¹ novalgin sample. A typical analytical procedure, including sampling and washing, could be performed in 1 min at a flow rate of 2.0 ml min⁻¹, giving a throughput of 60 h⁻¹. The proposed procedure was applied successfully in pharmaceutical preparations and furthermore the monitoring of novalgin in human urine without any pre-treatment process during 10 h. It was found that the novalgin concentration reached its maximum after orally administrated for about 4 h, and the novalgin metabolism ratio in 10 h was 10.83% in the body of volunteers. The flow system offered reagentless procedures and remarkable stability in determination of novalgin, and could be easily reused over 600 times.     

Determination of ultra-trace levels of cobalt by ion chromatographic separation and chemiluminescence detection

A luminol chemiluminescence detection/flow injection analysis technique coupled with ion chromatography (IC) has been examined for the selective determination of cobalt (II) at pg ml^?1 levels. A barium chloride solution was used as an eluent in the IC to separate cobalt(II) from interferents. When a 100-μ1 sample injection volume was used, the detection limit was 1.0 pg ml^?1 cobalt; the minimum detectable amount of cobalt was 100 fg. The calibration graph was linear above 10 pg ml^?1 and the linear dynamic range extended over six orders of magnitude. The relative standard deviation for ten replicate measurements of 30 pg ml^?1 cobalt was 3.8%. The results of the analysis of a synthetic sample corresponding to a boiling-water reactor coolant and some commercially available copper(II) standard solutions are given.     

Determination of ultra-trace rare earth elements in chondritic meteorites by inductively coupled plasma mass spectrometry

A method for the direct determination of ultra-trace rare earth elements (REE) in seven Chinese chondritic meteorites by inductively coupled plasma mass spectrometry (ICP-MS) was developed. Samples were digested with a mixture of HF+HNO₃ acids in Teflon pressure bomb. The accuracy and precision of the method were assessed by the analysis of four standard reference materials including one chondrite (Allende) and three basalts (BCR-1, BHVO-1 and W-2), the results obtained in this study agree quite well with the recommended values. The reproducibilities (expressed as RSD) of samples were less than 5%.     

Monolayers of human serum albumin

Summary The influence of different factors on the spreading of human serum albumin films is studied; factors such as the ionic strength of the spreading solution, nature and concentration of the alcohol used as spreading agent, initial spreading area of the subsolution to which the protein solution was applied and the method for the spreading (direct orTrurnit). The results obtained show that the ideal spreading solution is the buffer ph=5.1,=0.01, containing 0.5% amyl alcohol (v:v). TheTrurnit's method of spreading proteins showed significant advantage over the direct deposit of drops of the protein solutions.     

Voltammetric immunoassay of human albumin and goat antiserum to human albumin by nickel labeling

Summary Homogeneous und heterogeneous (in which globulin proteins were precipitated) voltammetric immunoassay (VIA) of nickel labeled human albumin was studied by monitoring the change in reduction currents of the metal protein complex. The concentration of human albumin nickel complex can be used to determine antiserum concentrations via immunochemical reaction. Concentration levels as low as 5.3×10^–7M goat antiserum to human albumin were measured using homogeneous VIA, and 3.3×10^–7 M using heterogeneous VIA and continuous flow analysis.

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Voltammetrische Immunoassay von Humanalbumin and Ziegenantiserum gegen Humanalbumin durch Nickelmarkierung

Zusammenfassung Ein homogener und ein heterogener (Fällung der Globulinproteine) voltammetrischer Immunoassay (VIA) von Nickelmarkiertem Humanalbumin wurde durch Messung der Änderung der Reduktionsströme des Metallproteinkomplexes untersucht. Die Konzentration des Humanalbumin-Nickelkomplexes kann zur Bestimmung von Antiserumkonzentrationen über eine immunochemische Reaktion benutzt werden. Konzentrationen bis herab zu 5,3·10^–7M Ziegenantiserum gegen Humanalbumin wurden mit dem homogenen VIA bestimmt, bis zu 3,3·10^–7M mit dem heterogenen VIA in Form der Durchflußanalyse.