微渗析活体取样—NiHCF修饰电极色谱电化学检测的研究

研究了六氰合亚铁酸镍修饰电极对单胺类递质及其代谢产物的催化机理，首次以该电极为色谱电化学检测器，对８种物质进行了分离测定，同时，半微渗析活体取样技术与高效液相色谱－电化学检测联用测定ＳＤ大鼠脑尾核处的单胺类递质及其代谢产物，并研究了Ｃａ＾２＋浓度对脑中递质的影响，拓展了电分析化学在生物活体分析中应用范围。     

高效液相色谱—电化学检测法测定大鼠脊髓灌流液单胺类递质及其代谢产物

用反相离子对高效液相色谱－电化学检测法分离并同时测定了大鼠脊髓灌流液中部分单胺类神经递质及其代谢产物。选择了较为理想的色谱条件，使生物样品的检测限达到８０～６７０ｐｇ，单胺类递质代谢产物的回收率保持在８３％～１０６％范围内。     

过氧化聚吡咯膜修饰电极色谱电化学用于帕金森试验动物的研究

研制了一种新型的过氧化聚吡咯膜修饰电极（OPPy/CME)作为液相色谱电化学检测器,该电极可以用来检测生物体内的单胺类神经递质及其代谢产物。用药物建立了帕金森动物试验模型,对不同情况下的试验动物脑内单胺类神经递质及其代谢产物通过微渗析取样和液相色谱电化学检测联用技术进行了测定。初步探讨了试验动物产生帕金森病的机理,为研制和筛选更有效的治疗帕金森病的新药提供了一种准确、可靠的分析手段。     

生物样本中单胺类递质及其前体氨基酸和主要代谢产物的快速分析法—高效液相色谱-电化学检测法

近年兴起的高效液相色谱-电化学检测法(HPLC-ECD)测定生物样本中单胺类递质,除了具有灵敏、快速、简便等优点外。同时还可以一次性分析单胺类递质及其前体氨基酸和主要代谢产物。我们结合本室条件,用HPLC-ECD法,同时测定生物样本中单胺类递质:去甲肾上腺素(NE)、肾上腺素(E)、多     

掺铈纳米二氧化铅修饰电极色谱电化学用于单胺类神经递质的研究

研制了一种新型掺铈纳米二氧化铅修饰电极，用X射线衍射（XRD）和扫描隧道 显微镜（STM）进行了表征。该修饰电极对单胺类神经递质及其代谢产物有良好的 电催化作用，灵敏度高，稳定性和重现性好，将其作为电化学检测器与液相色谱和 微渗析技术联用，测定了帕金森氏症病人脑脊液中单胺类神经递质及其代谢产物的 含量。取得了满意的结果并初步探讨了帕金森氏症的致病机理。     

碳纳米管/聚吡咯修饰电极用于液相色谱测定帕金森大鼠脑中神经递质

制备了碳纳米管/聚吡咯复合修饰电极,研究了多巴胺等单胺类神经递质在该修饰电极上的电化学行为.将此修饰电极作为电化学检测器,与高效液相色谱联用,测定了脑中7种神经递质及其代谢产物.结果表明:去甲肾上腺素、肾上腺素、多巴胺和5-羟色胺的线性范围为5.0×10(-10)～1.0×10(-5)mol/L;3,4-二羟基苯乙酸,...     

掺铂／聚3-甲基噻吩修饰电极研究氨酪酸对大鼠脑纹状体中单胺类神经递质影响

氨酪酸(GABA)是哺乳动物中枢神经系统中重要的抑制性神经递质.本研究探讨了外源性GABA对单胺类神经递质及其代谢产物的影响.研制了一种新型掺铂/聚3-甲基噻吩玻碳修饰电极,利用原子力显微镜(AFM)对该电极进行了表征,通过循环伏安法(CV)和微分脉冲伏安法(DPV)研究了单胺类神经递质及其代谢产物在该修饰电极上的电化学行为,结果表明:该修饰电极对单胺类神经递质及其代谢产物有显著的催化作用,电极的灵敏度高,稳定性和重现性好.在液相色谱电化学检测实验中,去甲肾上腺素(NE)、多巴胺(DA)、3,4-二羟基苯乙酸(DOPAC)、5-羟色胺(5-HT)和5-羟吲哚乙酸(5-HIAA)在修饰电极上的电流响应灵敏.5种被测物的检测线性范围宽达3个数量级以上,检出限分别为2.0×10-10 mol/L(NE)、1.0×10-10 mol/L(DA)、3.0×10-10 mol/L(DOPAC)、4.0×10-10 mol/L(5-HT)和7.0×10-10 mol/L(5-HIAA).将该方法与微渗析活体取样技术联用,研究了GABA对大鼠脑纹状体中单胺类神经递质及其代谢产物的影响.     

四氢生物蝶呤对大鼠纹状体中单胺类神经递质影响的液相色谱-电化学检测研究

四氢生物蝶呤(BH4)是生物体内单胺类神经递质合成过程中所需要的一种重要辅酶. 文中以Pt-Pd纳米修饰电极作为液相色谱电化学检测器, 采用高效液相色谱-电化学检测和微渗析活体取样技术, 研究了外源性的四氢生物蝶呤对大鼠纹状体中单胺类神经递质的影响. 研究表明外源性的BH4能提高大鼠纹状体中单胺类神经递质多巴胺(DA)、5-羟色胺(5-HT)及其代谢产物5-羟吲哚乙酸(5-HIAA)和高香草酸(HVA)的含量, 并进行了药物动力学分析, 探讨了BH4和单胺类神经递质浓度与时间的变化, 为一些神经疾病的病理学、药理学研究提供了新的分析手段.     

四氢生物蝶呤对大鼠纹状体中单胺类神经递质

四氢生物蝶呤(BH₄)是生物体内单胺类神经递质合成过程中所需要的一种重要辅酶. 文中以Pt-Pd纳米修饰电极作为液相色谱电化学检测器, 采用高效液相色谱-电化学检测和微渗析活体取样技术, 研究了外源性的四氢生物蝶呤对大鼠纹状体中单胺类神经递质的影响. 研究表明外源性的BH₄能提高大鼠纹状体中单胺类神经递质多巴胺(DA)、5-羟色胺(5-HT)及其代谢产物5-羟吲哚乙酸(5-HIAA)和高香草酸(HVA)的含量, 并进行了药物动力学分析, 探讨了BH4和单胺类神经递质浓度与时间的变化, 为一些神经疾病的病理学、药理学研究提供了新的分析手段.     

高效液相色谱法测定动物脑和脊髓内微透析样品中的递质氨基酸和单胺类递质及其代谢产物

 测定了猴、兔的尾核、海马和小脑深核以及猫脊髓背角微透析样品中递质氨基酸和单胺类递质及其代谢产物的含量。浓度与响应的线性关系、检测极限和重复性均与以前的报道一致。对应用常规液相色谱方法分析脑内微透析样品中的上述化合物时应注意的问题作了扼要的讨论。     

微柱液相色谱-双电极电化学法测定脑微透析液中单胺类递质的含量

用微柱液相色谱－双工作电极电化学检测法,分析了麻醉大白鼠纹状体微透析样品中的单胺类递质及其代谢产物的含量。无论在上游的氧化电位或下游的还原电位进行检测,至少在２～２００ｐｇ范围内,浓度与响应的线性关系良好,检测极限可达１ｐｇ以下。对于检测的优点和需要注意的问题作了扼要的讨论。     

Electrophoretic separations of twelve phenothiazines and N-demethyl derivatives by using capillary zone electrophoresis and micellar electrokinetic chromatography with non ionic surfactant

We focused our work on the separation of phenothiazines that are important drugs used for the treatment of psychic diseases. For a better understanding of the metabolism of these solutes, we wanted to separate not only a mixture of 12 phenothiazines but also a mixture containing phenothiazines and their N-demethyl metabolites by capillary electrophoresis. Separations in capillary zone electrophoresis were performed using 3 x 10(-2) mol/L H3PO4 (pH 2.5) but the obtained resolutions were not entirely satisfactory especially with regard to phenothiazine -N-demethyl derivative pairs. To improve the obtained results, we have performed separations by using micellar electrokinetic chromatography. In this approach, we used a running electrolyte containing 3 x 10(-2) mol/L H3PO4 electrolyte (pH 2.5) and octaethylene glycol monododecyl ether (C12E8) as neutral surfactant. By introducing 2 x 10(-3) mol/L C12E8 in the electrolyte, 11 out of 12 phenothiazines have been baseline separated. With respect to the separation of a mixture containing 3 phenothiazines and their 3 demethyl derivatives, we obtained an excellent separation by using a running electrolyte prepared with 7.5 x 10(-4) mol/L C12E8 and 3 x 10(-2) mol/L H3PO4.     

高效液相色谱/电化学法测定大鼠血液和脑组织中单胺类物质的含量

建立了高效液相色谱／电化学检测法测定大鼠脑组织和血液中单胺递质及其代谢产物的方法。能同时测定去甲肾上腺素（NE）、肾上腺素（E）、3,4-二羟基苯乙酸（DOPAC）、多巴胺（DA）、高香草酸（HAV）、5-羟色胺（5-HT）,并能和内标3,4-二羟卞胺（DHBA）分离良好。本方法快速、简便,回收率为92％-105％,线性范围2．8-680ng／mL,检出限为0．05ng（S／N=3）。本方法已应用在服用中药的大鼠下丘脑组织及血液的测定中,数据显示,本法能满足测定要求。     

高效液相-电化学检测法研究针刺对家兔血浆及脑组织中单胺类神经递质的影响

 通过高效液相 电化学检测法测定了电针刺激家兔肾旁穴前后其血浆及脑组织中单胺类神经递质去甲肾上腺素 (NE)、肾上腺素 (E)、多巴胺 (DA)和 5 羟色胺 (5 HT)含量的变化 ;研究了神经递质的变化与家兔繁殖能力的关系。该实验采用ODS柱 ,流动相为V(0 0 2mol/L柠檬酸三钠 0 0 5mol/L磷酸氢二钠 )∶V(甲醇 ) =95∶5的溶液 ,用电化学检测器检测。实验证明 ,血浆及脑组织中NE ,E ,DA和 5 HT的含量在针刺肾旁穴前后都有了显著的变化 ,说明针刺能激发家兔脑内神经元的活动 ,导致相应的递质含量的变化 ,同时使得血浆中相应含量也发生变化。     

四种阴离子的毛细管电泳电导检测(英文)

 采用柠檬酸 柠檬酸钠作为缓冲体系 ,使用负高压 ,对Cl-,NO3 -,HCO3 -和H2 PO4 -等 4种常见阴离子进行了分离检测 ,研究了缓冲剂的种类、浓度、pH值及操作电压对分离的影响。在选定的条件下 ,4种离子的定量线性范围 :Cl-5 0× 10 -5mol/L～ 2 5× 10 -3 mol/L ,NO3 -6 0× 10 -5mol/L～ 2 0× 10 -3 mol/L ,HCO3 -5 0× 10 -6mol/L～ 2 0× 10 -4 mol/L ,H2 PO4 -6 0× 10 -5mol/L～ 1 0× 10 -3 mol/L ;检出限 :Cl-1 5× 10 -5mol/L ,NO3 -3 0×10 -5mol/L ,HCO3 -1 0× 10 -6mol/L ,H2 PO4 -2 0× 10 -5mol/L ;峰面积的RSD (n =6 ) :Cl-3 1% ,     

新型安培检测毛细管电泳微系统

将电极、６ｃｍ分离毛细管、缓冲池、检测池集成于８．４×５．０ｃｍ有机玻璃片上,制作了一个毛细管电泳微系统。以碳纤维微盘电极作为工作电极,采用三电极体系柱端检测了１×１０－４ｍｏｌ／Ｌ多巴胺（ＤＡ）,具有良好的重现性,检测限３．６×１０－８ ｍｏｌ／Ｌ,线性范围５×１０－７～１×１０－４ｍｏｌ／Ｌ,并在该系统上分离了邻苯二酚（ＣＡ）和多巴胺的混合物。     

Simultaneous determination of monoamine transmitters, precursors and metabolites in a single mouse brain

A simple and sensitive procedure for simultaneous determination of monoamine transmitters and related substances including precursors and metabolites has been developed for a single mouse brain. The proposed procedure involves (1) primary butanol extraction, (2) separation of the substances into either acid or alkaline aqueous layers according to their physicochemical properties, and (3) determination by means of high-performance liquid chromatography with electrochemical detection. Three transmitters (noradrenaline, dopamine and 5-hydroxytryptamine) and their precursors (tyrosine, 3,4-dihydroxyphenylalanine and tryptophan) and major metabolites (normethanephrine, 3-methoxy-4-hydroxyphenylethylene glycol, 3-methoxytyramine, 3,4-dihydroxyphenylacetic acid, 3-methoxy-4-hydroxyphenylacetic acid and 5-hydroxyindoleacetic acid) were selectively separated and sensitively detected in mouse whole brain sample. Although 3-methoxy-4-hydroxymandelic acid was also separated from other substances by authentic chromatography, the substance was not detected in mouse brain. Changes in levels of these substances were examined for drugs whose effects had been previously confirmed. These changes reflected putative effects of the drugs and confirmed that the procedure is effective for neurochemical research into the transmitter system.     

Enantioselective analysis of pheniramine in urine by charged CD-mediated CZE provided with a fiber-based DAD and an on-line sample pretreatment by capillary ITP

Application potentialities of CZE on-line coupled with capillary ITP and DAD to the identification and determination of trace concentration levels (microg/L) of pheniramine (PHM) enantiomers and their metabolites present in complex ionic matrices of biological origin (urine) are shown. An enhanced (enantio)selectivity of the CZE separation system obtained by the addition of carboxyethyl-beta-CD (CE-beta-CD) to the carrier electrolyte provided CZE conditions for a reliable identification of similar/identical DAD spectra of structurally related compounds (PHM enantiomers and their metabolites) in clinical urine samples differing in qualitative and quantitative composition of sample matrix constituents. A high sample loadability (a 30 microL sample injection volume), partial sample clean-up (removing macroconstituents from the sample), and preconcentration of the analytes in ITP stage resulted in the decrease of concentration LOD for PHM enantiomers in urine to 5.2 and 6.8 microg/L (2.2 x 10(-8) and 2.8 x 10(-8) mol/L), without using any sample pretreatment technique. The background correction and smoothing procedure applied to the raw DAD spectra provided analytically relevant DAD spectra of PHM enantiomers and their metabolites also when they were present in urine sample (30 microL injection volumes of ten-times diluted urine sample) at a 9 x 10(-) (8) mol/L concentration. DAD spectra of PHM enantiomers present in urine samples matched their reference spectra with reasonable certainties. DAD spectra of PHM metabolites were compared with the reference spectra of PHM enantiomers and a good match was found which indicates the similarities in the structures of enantiomers and their metabolites detected in the urine samples. This fact allows performing the quantitative analyses of PHM metabolites in the urine samples by applying the calibration parameters of PHM enantiomers also for PHM metabolites and the results show the possibilities of using the ITP-CZE-DAD combination for the direct analysis of PHM enantiomers and/or their metabolites in urine without any sample pretreatment. ITP-CZE-DAD method with oppositely charged selector is suggested to use in clinical research as it provides favorable performance parameters including sensitivity, linearity, precision, recovery, and robustness with minimal demands on sample preparation.     

基于拮抗作用检测除草剂的类囊体膜生物传感器研究

利用除草剂对植物类囊体束缚酶分解过氧化氢的拮抗作用,研制了一种快速检测痕量除草剂的电化学生物传感器.将植物类囊体用聚乙烯醇-苯乙烯吡啶(PVA-SbQ)光敏聚合剂在紫外光诱导下产生大分子网状结构进行包埋,制成生物敏感膜,并固定在铂电极表面.根据加入除草剂时类囊体膜束缚酶分解过氧化氢活性的变化,对除草剂进行测定.在含有1×10^-3mol/LNaCl,5×10^-3mol/LMgCl₂和0.01mol/LH₂O₂的Tris-HCl缓冲溶液(pH=7.4)中,基于测量0.65V处H₂O₂氧化电流的变化,可以对下列浓度的除草剂进行定量检测:百草枯3×10^-9～1.5×10^-7mol/L,敌草龙1×10^-8～3×10^-7mol/L,扑草净4×10^-8～3×10^-6mol/L,阿特拉津1×10^-7～5×10^-6mol/L,莠灭净1×10^-7～5×10^-6mol/L.利用PVA-SbQ光聚合膜固定类囊体,能够使酶的活性在低温下保持数月.