以卡托普利为模板银纳米团簇的制备及生物硫醇的检测研究

生物硫醇在生物体内的代谢过程中起着重要作用,如体内半胱氨酸(Cys)和谷胱甘肽(GSH)含量异常会引发一系列疾病。为了建立一种快速、定量检测生物硫醇的荧光分析方法,本文以卡托普利(Captopril, Capt)为模板,采用湿化学还原法成功合成了发红色荧光的银纳米团簇(Capt-AgNCs),对Capt-AgNCs的形貌、结构、元素组成和光学性能等进行了表征。基于生物硫醇小分子对Capt-AgNCs的荧光猝灭作用建立了定量检测Cys和GSH的新方法,在最佳实验条件下,Cys和GSH的线性范围分别为1～100μmol/L和2～180μmol/L,检出限分别为0.054μmol/L和0.23μmol/L。该方法可用于人血浆中Cys的测定,回收率为95.3%～103.3%。实验结果表明,Capt-AgNCs作为一种新型信号关闭荧光探针,可用于Cys和GSH等生物硫醇的检测。     

新型磁性纳米金修饰过氧化氢生物传感器的研制

利用共沉淀法合成纳米Fe3O4颗粒,将半胱氨酸吸附到纳米Fe3O4微粒表面,借助半胱氨酸的巯基(-SH)对纳米金的强烈吸附,使纳米金自组装到磁性颗粒上,再通过静电吸附作用自组装辣根过氧化酶(HRP),合成了Fe3O4/Cys/Au/HRP纳米复合粒子,最后通过磁力将其修饰到固体石蜡碳糊电极表面,制得新型过氧化氢生物传感器.以对苯二酚作为电子媒介,用计时电流法对H2O2进行测定,线性范围为2.4 X10-3～6.0×10-6mol/L,检出限(S/N=3)为2.5 X 10-6mol/L,响应时间小于10 s.磁性纳米微粒Fe3O4/Cys/Au能够高效地保持HRP的生物活性.该新型传感器已用于实际样品测定.     

微渗析-液相色谱电化学检测法测定全血中的半胱氨酸和谷胱甘肽

采用微渗析取样作为样品预处理技术,与高效液相色谱电化学检测联用,建立了一种测定血中半胱氨酸(Cys)和谷胱甘肽(GSH)的新方法。电化学检测以玻碳电极为工作电极,结果表明在3.5×10-6～1.0×10-3mol/L浓度范围内,Cys和GSH的浓度分别与氧化峰的峰电流呈良好的线性关系,线性相关系数分别为0.9971和0.9982,检测限分别为1.2×10-6mol/L和3.2×10-6mol/L。     

毛细管电泳-电化学检测法测定血浆中水溶性小分子抗氧化剂

应用毛细管电泳电化学检测方法,以金属铜电极为检测电极,研究了同时测定人血浆中水溶性小分子抗氧化剂谷胱甘肽(GSH)、尿酸(UA)、色氨酸(Try)和半胱氨酸(Cys)的最佳条件。在最佳实验条件下,各组分的线性范围在1.0×10-6～5.0×10-4mol/L内;检出限在10-6mol/L数量级。该法具有分析速度快、灵敏度高等优点,对血浆样品的测定取得了满意的结果。     

2-硫代巴比妥酸修饰金纳米探针高灵敏比色检测三聚氰胺

以2-硫代巴比妥酸(TBA)修饰金纳米粒子为探针,TBA与三聚氰胺通过氢键作用诱导金纳米探针团聚,进而使金纳米胶体颜色由酒红色变为蓝色。 实验优化得最佳反应条件为在乙酸缓冲溶液（pH=7.0）介质中,室温反应15 min。 对不同浓度三聚氰胺进行检测时发现,在0.062~0.18 μmol/L和0.18~6.0 μmol/L之间,A660/A520吸收比率与三聚氰胺浓度呈现良好的线性关系,检出限为0.043 μmol/L。 该方法用于检测牛奶样品中的三聚氰胺的加标回收率为102.8%～105.3%。     

基于金纳米粒子自组装的分光光度法测定半胱氨酸

在pH 4.56的B ritton-Rob inson(B-R)缓冲溶液中,半胱氨酸的SH和NH3 分别与金纳米粒子表面进行共价结合和静电作用,导致金纳米粒子的长距离自组装,形成网状超分子结构,并使金纳米粒子的最大吸收波长从520 nm红移到660 nm。本实验对半胱氨酸引导的金纳米粒子自组装的作用机制进行了研究,建立了操作简便、高灵敏度测定半胱氨酸的分析方法。其线性范围为0.01~0.20 mg/L;检出限为2.8μg/L(3,σ2.3×10-8mol/L)。在实验条件下,其它常见的氨基酸和谷胱甘肽均不干扰测定。     

改性纳米金富集-毛细管电泳电化学发光法测定水产品中4种氟喹诺酮类药物残留

建立了一种利用改性纳米金粒子富集与毛细管电泳-电化学发光(CE-ECL)法测定水产品中4种氟喹诺酮(环丙沙星、恩诺沙星、氧氟沙星、诺氟沙星)类药物残留的分析方法。实验考察了富集条件与CE分离条件,并基于增强Ru(bpy)23+电化学发光的原理,优化了ECL检测条件。结果表明,在最优条件下,经改性金纳米粒子富集后的4种分析物在0. 05～10. 0μmol/L浓度范围内,其峰高与浓度呈现良好的线性关系,检出限(S/N=3)可达0. 2μmol/L,4种目标物的富集倍数达104～127倍。该方法用于鳗鱼样品的分析,回收率为94. 5%～112%,相对标准偏差(RSD)均不大于6. 3%。     

一种基于硝基烯烃的硫醇荧光探针的合成及生物成像研究

生命体内小分子硫醇,如半胱氨酸(Cys)、同型半胱氨酸(Hcy)和谷胱甘肽(GSH),在多种生理和病理过程中发挥重要作用.以氟硼二吡咯(BODIPY)为荧光团,硝基烯烃为识别基团,经三步简单有机合成,构建了一个打开型硫醇荧光探针.密度泛函理论计算结果表明,硝基通过光诱导电子转移(PET)机制淬灭BODIPY荧光.光谱测试结果表明,探针与硫醇发生迈克尔加成反应,响应迅速,选择性好,灵敏度高,对GSH的检测极限低至11×10~(-9) mol/L.荧光共聚焦成像结果表明,探针可用于HeLa细胞和斑马鱼内源生物硫醇荧光成像研究.     

碳纳米管修饰电极用于-高效液相色谱对全血中巯基化合物的测定

研究了羧基化多壁碳纳米管修饰电极 (MWNT CME)的制备方法和该修饰电极对巯基化合物的电催化行为 ,并首次以该修饰电极为电化学检测器 ,与高效液相色谱 (HPLC)联用 ,分离检测了半胱氨酸 (L Cys)和谷胱甘肽 (GSH)两种巯基化合物。结果表明在 3 .0× 1 0 - 7～ 1 .0× 1 0 - 3mol L浓度范围内 ,L Cys和GSH的浓度分别与其氧化峰的峰电流呈良好的线性关系 ,线性相关系数分别为 0 .9987和 0 .9990 ;检出限分别为 1 .2×1 0 - 7mol L和 2 .2× 1 0 - 7mol L。将该方法用于人全血中L Cys和GSH的测定 ,获得了满意的结果 ,为电分析化学在临床医学、生理学等生命科学中的应用提供了新的手段     

L-半胱氨酸自组装膜修饰金电极对抗坏血酸的电催化作用及其测定

金电极表面对L 半胱氨酸 (L Cys)有特性吸附 ,而L Cys分子在等电点pH附近因静电引力和氢键作用形成分子对 ,从而在电极表面自组装形成L Cys双层膜。L Cys修饰金电极对抗坏血酸 (AA)具有良好的电催化作用。用示差脉冲伏安法对AA进行了测定 ,氧化电流与AA的浓度在 1.0× 10 -3 ～ 4× 10 -6mol/L范围内呈良好的线性关系 ,线性相关系数为 0 .9981;检出限为 4× 10 -7mol/L。用于药片中AA含量的测定 ,结果令人满意。     

Nonionic surfactant‐capped gold nanoparticles for selective enrichment of aminothiols prior to CE with UV absorption detection

In this study, we describe the use of Tween 20‐capped gold nanoparticles (AuNPs) as selective probes for the extraction of aminothiols from an aqueous solution. Tween 20 molecules noncovalently attached to the surface of AuNPs to form Tween 20–AuNPs were used for the selective extraction of aminothiols through the formation of Au–S bonds. After extraction and centrifugation, the aminothiols were detached from the surface of the AuNPs by adding DTT in a high concentration. We used this probe in combination with CE and UV absorption detection. On‐line concentration and separation of the released aminothiols were performed by using 1.6% v/v poly(diallyldimethylammonium chloride) as an additive in CE. Under optimal extraction and stacking conditions, the LOD at a S/N of 3 were 28, 554, and 456 nM for glutathione (GSH), cysteine (Cys), and homocysteine (HCys), respectively. In comparison with the normal injection without the extraction procedure, approximately 2280‐, 998‐, and 904‐fold improvements in the sensitivity were observed for GSH, Cys, and HCys, respectively. We have validated the application of our method on the basis of the analysis of GSH and HCys in human urine samples. It is believed that this approach has significant potential to be extended to clinical diagnosis.     

An improved method for simultaneous analysis of aminothiols in human plasma by high-performance liquid chromatography with fluorescence detection

Altered levels of aminothiols in biological fluids are thought to be an important risk indicator for several diseases, and reliable methods for the accurate determination of aminothiols concentrations in plasma are thus required. In this paper ammonium 5-bromo-7-fluorobenzo-2-oxa-1,3-diazole-4-sulphonate (SBD-BF) is proposed as a convenient fluorogenic derivatizating reagent for the determination of aminothiols (cysteine, cysteinylglycine, homocysteine and glutathione) by HPLC with fluorescence detection. The reactions of SBD-BF with aminothiols at room temperature are about three-times faster than those of ammonium 7-fluorobenzo-2-oxa-1,3-diazole-4-sulphonate (the most frequently employed reagent) at 60 °C. The derivatives of SBD-BF with cysteine, cysteinylglycine, homocysteine and glutathione are easily separated by HPLC and their calibration curves show excellent linearity over the range 0.05–20 μmol/L with excellent r² values for all analytes. SBD-BF reacts with thiols under mild conditions, i.e. at 25 °C over about 30 min, and is proposed as a suitable fluorogenic reagent for thiol derivatization to be introduced in analytical clinical chemistry. The detection limits of Cys, Cys-Gly, Hcy and GSH at a signal-to-noise ratio of 5 were 0.1 μM for Cys, 0.01 μM for Cys-Gly and Hcy, and 0.02 μM for GSH. Furthermore, validation parameters of the proposed method are quite satisfactory. As an application of this method the determination of thiol derivatives in human plasma was carried out on a number of samples.     

Selective enrichment of aminothiols using polysorbate 20-capped gold nanoparticles followed by capillary electrophoresis with laser-induced fluorescence

In this article, we report a simple method for selective enrichment of aminothiols using Tween 20-capped gold nanoparticles (AuNPs) prior to capillary electrophoresis coupled with laser-induced fluorescence (CE-LIF). Compared to citrate-capped AuNPs, Tween 20-capped AuNPs exhibit the ability to disperse in a highly saline solution and selectively extract aminothiols through the formation of Au–S bonds. After extraction and centrifugation, 1 mM thioglycollic acid (TGA) was utilized to remove aminothiols that attached to the NP surfaces. After a solution of 8.0 mL aminothiols were extracted using 2× AuNPs (200 μL), the extracted aminothiols derivatized with o-phthalaldehyde at pH 12.0 were detected by CE-LIF. As a result, the limits of detection at a signal-to-noise ratio of 3 for homocysteine (HCys), glutathione (GSH), and γ-glutamycysteine (Glu-cys) are 4013.2, 79.8, and 382.8 pM, respectively. The use of this probe provided approximately 11-, 282-, and 21-fold sensitivity improvements for HCys, GSH, and Glu-cys, respectively. A practical analysis of HCys, GSH, and Glu-cys in human urine sample has been accomplished by this present method.     

在线衍生-高效液相色谱法同时测定血浆中的色氨酸及其代谢物

建立了醋酸锌在线衍生高效液相色谱法同时测定血浆中色氨酸(Trp)、犬尿氨酸(Kyn)、5-羟吲哚乙酸(5-Hiaa)和犬尿喹啉酸(Kyna)的方法。以3-硝基酪氨酸为内标(IS),采用Hypersil C-18柱(250 mm×4.0 mm, 5 μ m),以250 mmol/L醋酸锌溶液(pH 5.5)-乙腈(95:5, v/v)为流动相,流速为0.8 mL/min,柱温30℃。荧光检测波长设定:5-Hiaa为278 nm(λ_ex)/343 nm(λ_em), Kyna为244 nm(λ_ex)/400 nm(λ_em);紫外检测波长设定:Kyn和IS为360 nm, Trp为302 nm。4种物质的回收率在91.62%~114.17%之间;线性范围分别为2.50~320.00 μ mol/L(Trp), 0.32~15.36 μ mol/L(Kyn), 3.27~104.60 nmol/L(5-Hiaa), 14.00~464.80 nmol/L(Kyna);检出限分别为0.078 μ mol/L(Trp), 0.056 μ mol/L(Kyn), 0.690 nmol/L(5-Hiaa), 1.290 nmol/L(Kyna)。利用该方法对30例正常孕妇和28例女性健康志愿者的血浆进行测定,结果表明两组间Trp, Kyn和Kyna含量有显著性差异。该方法操作简便,重复性好,灵敏度高,适合于临床检测。     

HPLC-electrospray tandem mass spectrometry for simultaneous quantitation of eight plasma aminothiols: Application to studies of diabetic nephropathy

It was reported that Hcy was related to the development of kidney disease, but it remains unknown whether Hcy is an independent biomarker for diabetic nephropathy. Analytical method for simultaneous determination of aminothiols among the Hcy metabolic cycle is desirable to discover other potential biomarkers. A high-performance liquid chromatography-electrospray tandem mass spectrometric (HPLC-ESI-MS/MS) method was established for simultaneous quantitation of Cysteine (Cys), total homocysteine (tHcy), S-adenosylmethionine (SAM), S-adenosylhomocysteine (SAH), cystathionine (Cysta), methionine (Met), glutathione (GSH) and cysteinylglycine (Cys-gly) in plasma with N-(2-mercaptopropionyl)-glycine (MPG) as internal standard. The method had simple pretreatment without derivatization and the chromatograms show better separation of the eight aminothiols and the analytic time was 20 min. The results demonstrated that it provided an excellent linearity for all analytes over their respective concentration ranges and illustrated excellent precision and plasma recovery as well. Then, the method was applied in the case-control study of patients with diabetes mellitus (DM) and diabetic nephropathy (DN). In conclusion, it is an effective method to quantitate the concentrations of aminothiols in the human plasma. SAH and SAM were suggested as better potential biomarkers of DM and DN.     

亲水作用色谱法测定组织中全基因组DNA甲基化水平

建立了亲水作用色谱(HILIC)测定组织中全基因组DNA甲基化水平的方法。采用苯酚-氯仿提取组织中的DNA,提取的DNA用88%甲酸在140 ℃下裂解,经N2吹干后,加乙腈-水(9:1, v/v)溶解,用Waters BEH HILIC柱进行分离,在277 nm波长下检测胞嘧啶(Cyt)及5-甲基胞嘧啶(5-mCyt)含量。结果表明,以乙腈-10 mmol/L甲酸铵溶液(94:6, v/v)为流动相,流速为0.5 mL/min, Cyt与5-mCyt分离较好,保留时间分别为2.6与3.1 min。胞嘧啶的线性范围为1～900 μmol/L,相关系数为0.9999; 5-甲基胞嘧啶的线性范围为1～64 μmol/L,相关系数为0.9998。胞嘧啶和5-甲基胞嘧啶的检出限为54 nmol/L(柱中为0.54 pmol),定量限为250 nmol/L(柱中为2.5 pmol);在5～900 μmol/L的添加水平下,胞嘧啶和5-甲基胞嘧啶的平均加标回收率为94.7%～100.5%,相对标准偏差小于1.48%。用该方法检测了结肠癌组织中DNA甲基化水平,结果显示该癌组织中全基因组的DNA甲基化均值为4.0%。该方法快速、简单,稳定性好,灵敏度较高,能满足全基因组DNA甲基化的检测要求。     

以3,4-二羟基肉桂酸为介质的多壁碳纳米管糊电极用于检测药物和尿液样品中的谷胱甘肽(英文)

A sensitive and selective electrochemical sensor for the determination of glutathione(GSH) was developed using a modified multiwall carbon nanotube paste electrode with 3,4 dihydroxy cinnamic acid as a mediator.This modified electrode showed very high electrocatalytic activity for the anodic oxidation of GSH.Under the optimized conditions,the electrocatalytic peak current showed a linear relationship with GSH concentration in the range of 0.5-400.0 μmol/L with a detection limit of 0.1 μmol/L GSH.The relative standard deviations for seven successive assays of 5.0 and 25.0 μmol/L GSH were 2.2% and 2.7%,respectively.The modified electrode was used for the determination of GSH compounds in real urine samples.     

Amperometric determination of glutathione and cysteine on a Pd-IrO(2) modified electrode with high performance liquid chromatography in rat brain microdialysate

A Pd/IrO(2) co-electrodeposited glassy carbon electrode was prepared and the electrochemical behavior of glutathione (GSH) at this chemically modified electrode (CME) has been studied by cyclic voltammetry (CV). The results indicated that the modified electrode efficiently exhibited electrocatalytic oxidation for GSH with relatively high sensitivity, stability, and long-life. Coupled with high-performance liquid chromatography (HPLC), the Pd/IrO(2) modified electrode was utilized for the electrochemical detection (ECD) of the thiocompounds, glutathione and cysteine (Cys). The peak currents were linear with the substance concentrations in the range of 1.0 x 10(-5) mol L(-1) to 8.0 x 10(-4) mol L(-1) for GSH and 4.0 x 10(-6) mol L(-1) to 2.0 x 10(-4) mol L(-1) for Cys. The detection limits were 2.0 x 10(-6) mol L(-1) for GSH and 5.0 x 10(-7) mol L(-1) for Cys with S/N of 3. The method has been successfully applied to assess the contents of GSH and Cys in rat brain microdialysates.     

Hydroxyapatite nanoparticle prepared by controlled precipitation from aqueous phase

Hydroxyapatite nanoparticles (NPs) were prepared by controlled precipitation in the presence of stabilizers that confined growth and inhibited the aggregation of nanoparticles. Electrostatically stabilized NPs were prepared in the presence of sodium citrate; Tween 80 was used for steric stabilization. At low stabilizer concentrations, nanorods were formed of grown together, spheroidal hydroxyapatite NPs of ~20 nm in diameter. The rod length decreased as ether sodium citrate or Tween 80 concentration increased. When Cit^3–/Ca²⁺ = 3mol/mol, platelike NPs were formed 20–45 nm long and ~10 nm wide; for Cit^3–/Ca²⁺ = 4 mol/mol, NPs had sizes of 10–15 nm. At relatively high Tween 80 concentrations (>0.05 mol/L), foamlike structures were obtained.     

Detection of aminothiols through surface‐assisted laser desorption/ionization mass spectrometry using mixed gold nanoparticles

We have employed mixtures of two differently sized (average diameters: 3.5 and 14 nm) gold nanoparticles (Au NPs) as selective probes and matrices for the determination of aminothiols using surface‐assisted laser desorption/ionization mass spectrometry (SALDI‐MS). When using 38 and 150 pM solutions of the 3.5‐ and 14‐nm Au NPs, respectively, as the probe and matrix, SALDI‐MS provided limits of detection (signal‐to‐noise ratio = 3) of 2, 20, and 44 nM for 1.0 mL solutions of glutathione (GSH), cysteine (Cys), and homocysteine, respectively. The signal intensities of these analytes varied by less than 20% for SALDI‐MS analyses recorded over 50 sample spots; in contrast, they varied by as much as 60% when using a conventional matrix (2,5‐dihydroxybenzoic acid). We validated the practicality of this approach – with its advantages of sensitivity, reproducibility, rapidity, and simplicity – through the analysis of GSH in MCF‐7 cell lysates and Cys in plasma. Copyright © 2009 John Wiley & Sons, Ltd.