Colorimetric detection of glucose using a boronic acid derivative receptor attached to unmodifed AuNPs简

A simple, cheap and non-enzymatic colorimetric strategy for glucose detection has been designed based on the interactions between a phenylboronic acid （PBA） derivative, which is coupled with gold nanoparticles （AuNPs） as the colorimetric reporters, and glucose. The PBA-AuNPs hybrid system proposed here exhibits ordered photochemistry behaviors upon the addition of glucose at different pH values. There are two linear regions of glucose concentration for the glucose sensor at different pH values, i.e., between 0.1 mmol/L and 9.8 mmol/L at pH 6 with the detection limit of 64μmol/L and between 0 and 6.5 mmol/L with the detection limit of 48 μmol/L at pH 9, respectively. To test the practicality of the sensor system, we also applied this assay to detect a glucose sample in the artificial saliva.     

Study of blood collection and sample preparation for analysis of vitamin D and its metabolites by liquid chromatography–tandem mass spectrometry

The analysis of vitamin D status, with special emphasis on 25-hydroxyvitamin D and 1,25-dihydroxyvitamin D, is gaining interest in clinical studies due to the classical and non-classical effects attributed to this prohormone. In this research, the influence of the two steps preceding determination (viz. sample collection and preparation) on the quantitative analysis of vitamin D and its more important metabolites has been studied. Two preparation approaches, deproteination and solid-phase extraction (SPE), have been evaluated in terms of sensitivity to delimit their application, thus establishing that detection of 1,25-dihydroxyvitamin D cannot be addressed by protein precipitation. Concerning sample collection, serum and plasma reported high accuracy (above 83.3%) for vitamin D and metabolites, while precision, expressed as relative standard deviation, was below 12.9% for all analytes in both samples. Statistical analysis revealed that serum and plasma provided similar physiological levels for vitamin D₃, 24,25-dihydroxyvitamin D₃ and 25-hydroxyvitamin D₃, while significantly different levels were obtained for 1,25-dihydroxyvitamin D₃, always higher in plasma than in serum. Sample collection and treatment have proved to be significant in the analysis of vitamin D and its relevant metabolites.     

Resonance scattering spectral detection of ultratrace IgG using immunonanogold-HAuCl_4-NH_2OH catalytic reaction

Nanogold particles of 10 nm were used to label goat anti-human IgG (GIgG) to obtain nanogold-labeled GIgG (AuGIgG). In a citrate-HCl buffer solution of pH 2.27,AuGIgG showed a strong catalytic effect on the reaction between HAuCl4 and NH2OH to form big gold particles that exhibited a resonance scatter-ing (RS) peak at 796 nm. Under the chosen conditions,AuGIgG combined with IgG to form immuno-complex AuGIgG-IgG that can be removed by centrifuging at 16000 r/min. AuGIgG in the centrifuging solution also showed catalytic effect on the reaction. On those grounds,an immunonanogold catalytic RS assay for IgG was designed. With addition of IgG,the amount of AuGIgG in the centrifuging solution decreased; the RS intensity at 796 nm (I796 nm) decreased linearly. The decreased intensity ΔI796 nm was linear with respect to the IgG concentration in the range of 0.08-16.0 ng·mL-1 with a detection limit of 0.02 ng·mL-1. This assay was applied to analysis of IgG in sera with satisfactory sensitivity,selectivity and rapidity.     

一种基于纳米二氧化硅增强凝集反应的压电免疫传感器

本文提出了一种基于抗体包被纳米粒子的简单快速的压电免疫凝集法,用于蛋白质检测。该方法原理是利用羊抗人IgG（G-anti-hIgG）包被的二氧化硅（或金）纳米粒子和人IgG（hIgG）发生免疫凝集反应而使得压电晶体频率发生改变进行测定。当凝集反应发生时,修饰在探针表面的G-anti-hIgG通过hIgG与G-anti-hIgG包被的纳米粒子结合,将质量效应和粘弹性因素叠加作用于压电晶体。结果表明这使得背景值大幅减小而信号明显增强。另外,对修饰后了抗体及结合免疫复合物的探针表面进行了SEM表征,对使用聚乙二醇作为增敏剂和实验最佳离子强度、pH值进行了优化选择。该传感器检测hIgG线性范围是0.26-16.7 mg mL-1,最低检出限为84 ng mL-1。     

一种快速高选择性检测痕量癌胚抗原的共振散射光谱法

用10 nm的金纳米粒子标记单克隆癌胚抗原抗体制备了检测癌胚抗原（CEA）的共振散射光谱探针（Au-CEAAb）。在pH 6.8 的Na2HPO4- NaH2PO4缓冲溶液中及聚乙二醇-6000存在下, CEA与Au-CEAAb发生免疫反应聚集形成疏水性的、平均粒径为227.0 nm的免疫复合物微粒,并在321 nm、581 nm产生2个共振散射峰。随着癌胚抗原（CEA）浓度的增大,581 nm处的共振散射强度I581nm线性增加,其增加值△I581nm与CEA浓度在1.0～50.0 ng·mL-1范围内呈良好的线性关系,相应的回归方程、相关系数、检出限(3σ)分别为ΔI581nm=1.63 C +5.6、0.9940、0.52 ng·mL-1。该法简便、快速、灵敏且选择性好,用于检测人血清中癌胚抗原（CEA）,结果满意。     

Rapid and quantitative method for evaluating the personal therapeutic potential of cancer drugs

An in vitro, rapid, and quantitative cell-based assay is needed to predict the efficacy of cancer drugs in individual patients, because a cancer patient may have unconventional aspects of tumor development. Here we report a rapid and label-free quantitative method for verifying apoptosis in living cancer cells cultured on a sensor chip with a newly developed high-precision surface plasmon resonance (SPR) sensor. The time-course cell reaction was monitored as the SPR angle change rate for 5 min during a 35-min cell culture of pancreatic cancer lines with a drug. The time-course cell reaction was significantly related to cell viability counted after 48 h as assessed by caspase-3 activity assay of apoptosis. Furthermore, the detected SPR signal was derived from the decrease in inner mitochondrial membrane potential. The results obtained are universally valid for various cancer drugs mediating apoptosis through different cell-signaling pathways and even for combined use in various pancreatic cancer cell lines. This system can be applied in a clinical setting to evaluate the personal therapeutic potential of drugs including pharmacodynamic interactions.     

A multianalyte ELISA for immunochemical screening of sulfonamide,fluoroquinolone and ß-lactam antibiotics in milk samples using class-selective bioreceptors

A multianalyte ELISA has been developed for the simultaneous determination of the most frequently used antibiotic families in the veterinary field following the typical planar microarray configuration, where the identity of the target analyte is encoded by its location in the detection platform (Master et al. in Drug Discovery Today 11:1007-1011, 2006). To accomplish this aim, two individual enzyme-linked immunosorbent assays for sulfonamide and fluoroquinolone antibiotics and an enzyme-linked receptor assay for ss-lactam antibiotics have been combined. The strategy uses microplates coated with the corresponding haptenized proteins in specific sections of the microplate. The samples are mixed with a cocktail containing the bioreagents, and distributed in the wells of the microplate. Identification of the antibiotic present in a particular sample is consequently accomplished by detecting a positive response on the corresponding microplate section. Since the bioreceptors used show a wide recognition of the congeners of each antibiotic family, the multianalyte method is able to detect more than 25 different antibiotics from the three most important antibiotic families. The detectability reached in full-fat milk samples is below the European maximum residue limits. The accuracy and reliability of this multiplexed bioanalytical method have been demonstrated by analyzing blind spiked samples.     

硫酸分离–火试金重量法测定碲化铜中的金和银

建立了用硫酸分离-火试金重量法测定碲化铜中的金和银含量的方法。用硫酸溶解碲化铜样品,过滤,除去铜和碲,得到含金、银的沉淀物,沉淀物经灰化、配料、高温熔融制得铅扣。将铅扣灰吹,得到金银合粒,用硝酸溶解分离金,用重量法测定金含量。用金银合粒的质量扣除金粒的质量和分金液、洗液中杂质的质量即为银含量。采用灰皿、残渣熔融法补正,或用含碲、铜物料做基体加入纯金、纯银同试样方法测定,根据金、银的回收率加以补正,从而得到试样中的碲含量。实验结果表明,浓硫酸的加入量为30 mL,残余量应不少于15 mL。火试金中硅酸度为1左右,试样进炉温度以900℃为宜。该方法金、银测定结果的相对标准偏差分别为0.33%~1.97%,0.28%~1.27%(n=9)。金的回收率为98.5%~100.2%,银的回收率为95.5%~101.4%。该法满足生产控制检测和贸易结算的要求。