Enzyme-catalyzed reaction of OPD-H202-HRP voltammetric enzyme-linked immunoassay system

Enzyme-catalyzed reaction of o-phenylenediamine (OPD)-H_z0₂-horseradish peroxidase (HRP) voltammetric enzyme-linked immunoassay system has been studied in detail with electrochemical analysis, high performance liquid chromatography (HPLC), ultraviolet/visible (UV/Vis) spectroscopy, infrared (IR) spectroscopy and nuclear magnetic resonance (NMR) spectroscopy. The pure product of H₂0₂ oxidizing OPD catalyzed by HRP was prepared with chemical method. The experimental results of voltammetry and HPLC indicate that only one product of enzyme-catalyzed reaction has been obtained under the selected enzyme-catalyzed reaction conditions. Identifications by UV/ Vis spectrum, IR spectrum and¹³C NMR spectrum show that the product is 2,3-diaminophenazine. The processes of the enzyme-catalyzed reaction and the electroreduction of the product of the enzyme-catalyzed reaction are described. Project supported by the National Natural Science Foundation of China     

PAP-H2O2-HRP酶促反应产物光谱及电化学研究

前文［１］首次提出了以对氨基酚（ＰＡＰ）为底物的ＰＡＰ－Ｈ２Ｏ２－辣根过氧化物酶（ＨＲＰ）伏安酶联免疫分析新体系,并成功地应用于烟草花叶等植物病毒的血清学检测．在此之前,我们也曾报道过一些伏安酶联免疫分析新体系［２,３］．迄今,还没有人对 ＨＲＰ催化 Ｈ２Ｏ２氧化 ＰＡＰ的酶促反应进行过探讨．Ｐｒａｔｉ等［４］报道了在铜催化作用下,Ｏ２氧化对氨基酚生成３－［（４－个羟苯基）氨基」－４－（２－氨基－５－羟苯基）－６－［（４－羟苯基）亚胺基］－２,４－环己二烯基－１－酮．本文的实验结果与此文献不符． 为…     

Enzyme-catalyzed reaction of voltammetric enzyme-linked immunoassay system based on OAP as substrate

The o-aminophenol (OAP)-H_2O_2-horseradish peroxidase (HRP) voltammetric enzyme-linked immunoassay new system has extremely high sensitivity. HRP can be measured with a detection limit of 6.0×10~-(10) g/L and a linear range of 1.0×10~(-9)—4.0×10~(-6) g/L. The pure product of H_2O_2 oxidizing OAP catalyzed by HRP was prepared with chemical method. The enzyme-catalyzed reaction has been investigated with electroanalytical chemistry, UV/Vis spectrum, IR spectrum, ~(13)C NMR, ~1H NMR, mass spectrum, elemental analysis, etc. Under the selected enzyme-catalyzed reaction conditions, the oxidation product of OAP with H_2_O2 catalyzed by HRP is 2-aminophe-noxazine-3-one. The processes of the enzyme-catalyzed reaction and the electroreduction of the product of the enzymecatalyzed reaction have been described.     

MAP-H~2O~2-HPR伏安酶联免疫分析新体系和光谱及电化学研究

提出了间氨基酸(MAP)-H~2O~2-辣根过氧化物酶(HRP)伏安酶联免疫分析新体系.本方法以线性扫描二阶导数伏安法检测HRP催化H~2O~2氧化MAP的产物,用于游离HRP和各种HRP标记物的测定,灵敏度均高于经典的ELISA显色光度法.测定游离HRP的线性范围为1.0x10^-^8-1.0x10-6/L,检测限达3.8x10^-^9g/L.制备出了HRP催化H~2O~2氧化MAP的产物纯品并应用电化学分析,高效液相色谱,元素分析,紫外-可见光谱,红外光谱,^1H核磁共振谱,^1^3C核磁共振谱及质谱等技术对体系酶促反应进行了深入的研究.在选择的酶促反应条件下,生成的产物为2-氨基-5-[(3-差苯基)]-2,5-环己烯基-1,4-二酮.提出了酶催化反应机理及其产物的电极还原过程。     

预混合自组装辣根过氧化物酶生物活性膜及其催化活性研究

以阳离子化的辣根过氧化物酶 (HRP)和阴离子聚苯乙烯磺酸钠 (PSS)的预混合溶液 ,与阳离子聚电解质聚二甲基二烯丙基氯化铵 (PDDA)通过逐层组装 ,在阴离子化聚对苯二酸乙二酯 (PET)表面构建了多层生物活性膜 .用紫外 可见光谱仪 (UV Vis)和原子力显微镜 (AFM)研究了交替自组装膜的结构和表面形膜 ,并测定了自组装膜的生物催化活性 .结果表明 ,预混合溶液中的PSS与HRP一起沉积在PDDA膜层上组装成 (PSS+HRP)膜层 ,且每层中PSS和HRP的比例一致 ;(PSS +HRP)膜层呈条状分布 ,膜表面较为平整 ;多层膜中的HRP催化H2 O2 与 4 氨基安替比林的显色反应的表观米氏常数为 9 7× 10 - 5mol·L- 1 (相对于H2 O2 底物 ) ,较溶液中 (1 5 2× 10 - 4mol·L- 1 )的小 .     

生物酶HRP催化H~2O~2氧化间苯二胺反应的研究

应用电化学分析,高效液相色谱(HPLC),紫外-可见光谱(UV-vis),红外光谱(IR)和核磁共振(NMR)等技术对辣根过氧化物酶(HRP)催化H~2O~2氧化间苯二胺(MPD)的反应进行了研究。伏安法和高效液相色谱实验说明,在所选择的酶催化反应条件下,酶催化反应生成一种产物。用化学方法制得了HRP酶催化H~2O~2氧化MPD的产物纯品。经UV-vis,IR和^1HNMR谱鉴定,产物为2,7-二氨基吩嗪。写出了酶催化反应过程,同时对酶催化反应产物的电极还原过程也进行了研究。     

四铁取代的夹心型钨砷酸盐的合成及玻碳电极表面多层膜组装与电催化性质研究

碳电极表面的修饰在电化学和材料科学中很重要 .最近 ,通过层与层电子间的相互作用来自组装修饰玻碳电极已引起人们的关注 [1] .运用这种方法可将一些功能团修饰到电极表面 ,赋予电极一些新的功能 [2 ] .过渡金属取代的多金属氧酸盐不仅在配位环境 ,而且在催化活性方面都类似于金属卟啉和其它大环配体金属配合物 [3] .将其修饰到玻碳电极表面已有文献报道 [4 ] .由于修饰电极的厚度可控、成分可调及具有良好的电催化活性 ,在生物传感器和电子器件等方面具有潜在的应用前景 .取代型夹心型多金属氧酸盐具有大摩尔质量和高电荷密度 ,表现出优秀…     

微孔多酸CsxH5-xPW10V2O40/SiO2的制备及氧化催化作用

Keggin结构杂多酸在固相体系中的催化作用引起了人们的极大兴趣[1～3].性能稳定的杂多酸铯盐催化剂在非均相催化体系中已有广泛的应用,然而由于其在液固体系中通常呈现牛奶状,难以分离和重新使用,尽管化学家们以各种材料作为这些催化剂的载体进行了许多固载化尝试[4～6],但至今尚未从根本上解决这一难题.因此,开发高比表面的耐水微孔固体杂多酸催化剂是多酸催化化学领域中具有理论和实际意义的课题.本文采用Sol-Gel技术,以正硅酸乙酯(TEOS)为硅源,水解产生的具有网络结构的SiO2凝胶为载体,在钒取代型Keggin结构杂多酸CsxH5-xPW10V2O40存在下,制得通式为CsxH5-xPW10V2O40/SiO2的固体双功能微孔杂多酸; 以30%H2O2为氧化剂,以苯甲醇氧化为模型反应,研究其液-固体系中的催化作用.     

DNA与邻苯二胺-过氧化氢-过氧化物酶体系相互作用的光谱研究

用光谱方法研究了邻苯二胺－过氧化氢－过氧化物酶体系与ＤＮＡ的作用，认为二者之间发生的是嵌插作用。分别用ＵＶ－Ｖｉｓ光谱和荧光光谱求得了形成常数，两种方法具有一致性。讨论了ｐＨ值对嵌插作用的影响。     

过氧化物酶新型荧光底物3,4-二氢-2(1H)-喹喔啉酮的反应机理及性能的研究

合成了过氧化物酶新型荧光底物3,4-二氢-2(1H)-喹喔啉酮(DHQXL). 在过氧化物酶催化下,该化合物可被H₂O₂氧化生成强荧光物质2(1H)－喹喔啉酮(QXL). 用高压液相色谱法分离得荧光产物纯品,经核磁共振谱和质谱证实其结构,确证了提出的酶催化反应机理. 对该化合物作为荧光底物的性能研究表明,它是一个很有应用前景的过氧化物酶的新型荧光底物.     

(R)-2-{[4-(3-甲氧基丙氧基)-3-甲基吡啶-2-基]甲基亚硫酰基}- 1H-苯并咪唑的合成

以2,3-二甲基吡啶为起始原料, 经过11步反应, 不对称合成了质子泵抑制剂的关键中间体: (R)-2-{[4-(3-甲氧基丙氧基)-3-甲基吡啶-2-基]甲基亚硫酰基}-1H-苯并咪唑. 研究了用手性高效液相色谱拆分对映体、测定产品光学纯度的方法, 结果表明目标产品的ee值达到99%. 通过IR, UV, MS以及1H NMR分析对重要中间体和目标产品进行了结构鉴定.     

1,4-双氯甲基-2-甲氧基-5-壬氧基苯的均聚和共聚

以对甲氧基苯酚和溴壬烷为原料,经过醚化和双氯甲基化反应得到１,４－双（氯甲基）－２－甲氧基－５－壬氧基苯（ＢＣＭＮＯＮＯＢ）,ＢＣＭＭＯＮＯＢ在强碱作用下通过脱氯化氢得到可溶性的聚（２－甲氧基－５－壬氧基）对苯乙炔（ＰＭＯＮＯＰＶ）;首次采用脱氯化氢消除反应实现了ＢＣＭＭＯＮＯＢ与１,４－双（氯甲基）－２,５－二甲基（ＢＣＭＤＭＢ）共聚。讨论了两种单体结构和縻尔比率及溶剂因素对聚合反应和共聚物溶解     

Synthesis and structural characterization of the novel cluster compound

Reaction of [Mo3Y(mu-S)3(dtp)4(H2O)] (Y = O, S; dtp = S2P(OC2H5)2(-)) with HgI2 gave the novel compound [[Mo3S7(dtp)3]4 x I][(HgI3)3] x 4H2O (1), which contains a [[Mo3S7(dtp)3]4 x I] tetramer and (HgI3)-. Compound 1 has been characterized by IR, Raman, UV/Vis, and NMR spectroscopy and single-crystal X-ray diffraction analysis. It is shown that this formation process can be referred to as a new cluster reaction. The structure and spectroscopic data of the tetramer is also compared with that of the related discrete cluster [Mo3S7(dtp)3 x I]. Crystal data: space group F23, a = 26.786(3) A, V = 19218.7(4) A3, Z = 4, R = 0.059.     

邻苯二酚作螯合剂合成全硅方钠石(Si-SOD)和全硅ZSM-5(Si-ZSM-5)分子筛大单晶

通过在两个合成分子筛的体系SiO₂-NaOH-EG-R和SiO₂-TPABr-NaOH-H₂O-R(R:邻苯二酚,EG:乙二醇)中加入邻苯二酚获得了具有较大尺寸和完美形貌的分子筛单晶。²⁹SiNMR,IR和UV-Vis光谱表明,在反应混和物中有硅-邻苯二酚螯合物生成,这种硅的螯合物在形成分子筛大单晶过程中起到了缓释硅源的作用。     

KF/Al2O3催化下取代水杨醛与达米酮的反应

取代水杨醛与5,5-二甲基-1,3-环己二酮(达米酮)在KF/Al2O3催化下反应生成一系列苯并吡喃的衍生物.产物的结构通过红外光谱、核磁共振氢谱和元素分析进行表征,并通过X单晶衍射分析进一步证实产物的结构.     

Synthesis and magnetic,spectral and thermal eukaryotic DNA studies of some 2-acetylpyridine- [N-(3-hydroxy-2-naphthoyl)] hydrazone complexes

Complexes of Ni(II), Co(II), Cu(II), Zn(II), Cd(II), Hg(II) and U(VI)O₂ with 2-acetylpyridine-[N-(3-hydroxy-2-naphthoyl)] hydrazone (H₂APHNH) have been prepared and characterized by elemental analysis, molar conductance, thermal (TG, DTG), spectral (¹H NMR, IR, UV–Vis, ESR) and magnetic measurements. ¹H NMR spectrum of the ligand suggests the presence of intramolecular hydrogen bonding. IR spectra show that H₂APHNH is a bidentate, tridentate and/or tetradentate ligand. Thermal decomposition of some complexes ended with metal oxide as a final product. ESR spectra gave evidence for the proposed structure and the bonding for some Cu(II) complexes. Biological activity measurements were carried out.     

邻苯二胺产品中针状未知化合物的结构鉴定

从邻苯二胺产品中分离出一种白色针状未知化合物,用液相色谱（ＨＰＬＣ）和气相色谱（ＧＣ）鉴定其纯度后,同时进行元素、红外光谱（ＩＲ）、紫外光谱（ＵＶ）、质谱（ＭＳ）、核磁共振（ＮＭＲ）氢谱及碳谱分析。根据分析的结果进行解析,最后确定未知针状不纯物中其主成分为２,１,３－苯并硫咪唑或２,１,３－硫二氮杂茚（Ｃ６Ｈ４Ｎ２Ｓ）（２,１,３－ｂｅｎｚｏｔｈ－ｉａｄｉａｚｏｌｅ）。     

Synthesis and characterization of Hg(II) and Zn(II) complexes based on 3-[(4-chlorophenylamido)]propenoic acid

3-[(4-Chlorophenylamido)]propenoic acid has been synthesized by reaction of maleic anhydride and 4-chloroaniline in 1:1 molar ratio in glacial acetic acid and its metal complexes have been synthesized by the reaction of 3-[(4-chlorophenylamido)]propenoic acid with HgCl₂ and [Zn(CH₃COO)₂] · 2H₂O in 2: 1 molar ratio, respectively. All the synthesized compounds have been characterized by the elemental analysis, IR, UV/Vis and NMR (¹H, ¹³C) spectroscopy. Conductance for the reported compounds has been recorded in ethanol and suggests the non-electro lytic nature of complexes. IR data of metal complexes shows that the ligand is bound to the metal via both carboxylate oxygen atoms and complexes exhibits 4-coordinated geometry in solid state. NMR (¹H, ¹³C) study confirms the structure of the 3-[(4-chlorophenylamido)]propenoic acid and the reported complexes.     

Investigation of voltammetric enzyme-linked immunoassay based on a new system of HAP-H2O2-HRP

By introducing heterocyclic compound to immunoassay system as an electrochemical substrate for the fist time, a new voltammetric enzyme-linked immunoassay system of 3-hydroxyl-2-aminopyridine (HAP)-H(2)O(2)-horseradish peroxidase (HRP) has been developed. HAP was oxidized with H(2)O(2) catalyzed by HRP, and the resulting electroactive product produced a sensitive voltammetric peak at potential of -0.36 V (vs. SCE) in Britton-Robinson (BR) buffer solution. The process of the enzyme-catalyzed reaction and the electro-reduction of the product have been investigated in detail. The linear range for detection of free HRP was from 4.0x10(-13) to 1.0x10(-9) g/mL with a detection limit of 1.2x10(-13) g/mL. The new system has been successfully applied for the assay of alpha-fetoprotein (alphaFP) in human serum ranging from 0.1 to 200 ng/mL with a detection limit of 0.1 ng/mL, which was 10 times lower than that of traditional spectrophotometric enzyme-linked immunosorbent assay (ELISA) method. HAP-H(2)O(2)-HRP voltammetric enzyme-linked immunoassay showed a promising alternative approach in the detection of alphaFP in clinical diagnosis.     

Studies on the oxidation reaction of tyrosine (Tyr) with H2O2 catalyzed by horseradish peroxidase (HRP) in alcohol-water medium by spectrofluorimetry and differential spectrophotometry

An oxidation reaction of tyrosine (Tyr) with H(2)O(2) catalyzed by horseradish peroxidase (HRP) was studied by spectrofluorimetry and differential spectrophotometry in the alcohol(methanol, ethanol, 1-propanol and isopropanol)-water mutual solubility system. Compared with the enzymatic-catalyzed reaction in the water medium, the fluorescence intensities of the product weakened, even extinguished. Because the addition of alcohols made the conformation of HRP change, the catalytic reaction shifted to the side of polymerization and the polymer (A(n)H(2), n>or=3) exhibited no fluorescence. The four alcohols cannot deactivate HRP. Moreover isopropanol activated HRP remarkably.