2,4-二羟基苯乙酮缩异烟酰腙的实验和DFT理论研究:合成、晶体结构和性质及量化计算

合成了一种酰腙类Schiff碱2,4-二羟基苯乙酮缩异烟酰腙(C₁₄H₁₃N₃O₃,H₂L),经元素分析、红外光谱、紫外光谱、荧光光谱和热重分析等技术手段进行了表征。 用X射线单晶衍射测定了它的晶体结构,该晶体属单斜晶系,C2/c空间群,晶胞参数a=2.0102(2) nm,b=0.75891(8) nm,c=1.9530(2) nm,α= 90°,β=111.481(12)°,γ=90°,V=2.7725(5) nm³,Z=4,D_c=1.4292 g/cm³,R₁=0.0422,wR₂=0.1113,F(000)=1256。 同时进行了量子化学计算研究。 使用Gaussian09量子化学程序包, 在密度泛函理论(DFT)的B3LYP/6-31G(d)水平,对化合物的分子结构进行全参数优化计算,获得了热力学参数和几何结构参数,对分子的总能量及前线分子轨道、Mulliken电荷分布进行了分析讨论;同时,用TD-DEF方法计算了化合物的电子吸收光谱和荧光发射光谱。     

α,β,γ,δ,ε,η-Bi2O3电子结构和光学性质的第一性原理研究

基于密度泛函理论的CASTEP模块研究了α, β, γ, δ, ε和η-Bi₂O₃晶型, 计算分析了其几何结构、 能带结构、 电子态密度和光学性质. 结果表明, α, ε和η相均为层状结构, 其中, α和ε相为单层—Bi—O—结构, 而η相为双层—Bi—O—结构; β, γ和δ相为—Bi_m—O_n—交错结构, 其中δ相交错尤为密集, 呈现导体特性. 各晶相的导带均由Bi 6p态构成, 价带由O_2p态起主导作用. 电势电位分析结果表明, 6种晶相价带电位均在H₂O/O₂之下, 具有强氧化能力, 与实验报道的光催化氧化能力大小顺序γ-Bi₂O₃>β-Bi₂O₃>α-Bi₂O₃>δ-Bi₂O₃一致, 而导带还原电位低于H₂/H₂O, 预测纯Bi₂O₃很难具备催化产氢能力. 光学性质分析发现, γ和δ相的起始响应波长较大, 说明其应具备红外激发的性质. 这些结果可为获得偏红外激发和较宽光谱响应的Bi₂O₃材料研究提供理论基础, 为研发和应用Bi₂O₃及其复合物提供重要的指导.     

黑果枸杞叶多糖LRLP3的结构、抗氧化活性及免疫活性

黑果枸杞叶经水提醇沉, 离子交换柱层析和凝胶柱层析分离纯化, 得到平均分子量为79400的均一多糖组分LRLP3. 对该多糖的理化性质、 结构、 抗氧化活性及免疫活性的研究结果表明, LRLP3为多分支结构, 主链为(1→3)βGalp, 大部分半乳糖6位存在分支; 支链由(1→6)βGalp, (1→4)βGalp, (1→3)βAraf, (1→3)αArap, (1→5)βAraf和(1→2,4)αRhap组成, 非还原末端由αAraf, βGalp和βGlcp组成. LRLP3具有较强的还原能力, 可显著清除1,1-二苯基-2-三硝基苯肼(DPPH)自由基、 羟自由基和超氧阴离子自由基, 有效抑制Cu²⁺/H₂O₂诱导的蛋白氧化损伤和H₂O₂诱导的细胞氧化损伤. LRLP3在体外对未经诱导和经刀豆蛋白(ConA)或脂多糖(LPS)诱导的小鼠脾细胞增殖均有促进作用.     

一种新型钼钒多酸化合物的合成、结构与荧光性能

采用水热技术,合成了一种新型四帽Keggin结构多酸化合物[H₃Mo₈^ⅥV₈^ⅣO₄₀(AsO₄)](en)₂(4,4-bipy)₇·9H₂O(en:乙二胺;bipy:联吡啶)(1),并对化合物进行了元素分析、红外光谱、X射线光电子能谱和X射线单晶结构分析。 晶体结构分析表明, 化合物属三斜晶系,P1空间群,晶胞参数a=1.47395(5) nm,b=1.48172(6) nm,c=1.62881(7) nm,α=66.16(3)°,β=87.15(2)°,γ=63.42(1)°,V=2.8723(2) nm³,Z=1,R₁=0.0728,wR₂=0.2014。 化合物由四帽Keggin多酸阴离子、4,4'-联吡啶、乙二胺和结晶水分子构成,化合物分子间存在大量的氢键,使化合物1形成3-D超分子结构。 荧光测试表明,化合物1能发出较强的荧光,有可能成为潜在的光活性材料。     

亚磷酸锌无机-有机杂化化合物的合成与结构表征

在水热条件下, 以1,6-己二胺为模板剂合成了一个三维(3D)亚磷酸锌无机-有机杂化化合物(C₆N₂H₁₆)_0.5ZnHPO₃(ZnHPO-CJ15), 并对其单晶结构进行了解析. 结果表明, ZnHPO-CJ15晶体属单斜晶系, P2₁/c空间群, a=1.19587(7) nm, b=0.82766(5) nm, c=0.77756(5) nm, α=90.00°, β=95.8370(10)°, γ=90.00°, V=0.76562(8) nm³, Z=1. ZnHPO-CJ15具有层柱状结构, 其骨架结构是由ZnO₃N四面体和HPO₃假四面体连接构成的二维4×8元环网层结构, 层与层之间由1,6-己二胺分子与Zn配位柱撑连接形成三维结构.     

相转移催化合成黄豆黄苷的研究

以4-甲氧基间苯二酚和对羟基苯乙腈通过Hoesch反应制备的7,4'-二羟基-6-甲氧基异黄酮(黄豆黄素)为苷元,以三(3,6-二氧杂庚基)胺(TDA-1)为相转移催化剂,碳酸氢钠/氯化钾体系为碱性介质,研究了黄豆黄素与1-溴-2,3,4,6-O-四乙酰基-α-D-吡喃葡萄糖进行偶联反应制备大豆异黄酮黄豆黄苷的合成工艺,糖苷化反应收率为77%,结构经IR和1H NMR以及元素分析加以确证.     

基于二茂铁的两个查尔酮衍生物的合成及超快三阶非线性光学响应

二茂铁是合成新颖有机功能材料的基本单元之一。 本文设计并合成了两个基于二茂铁的同分异构查尔酮衍生物:1-二茂铁基-3-(噻吩-2-基)丙烯酮(a)和1-二茂铁基-3-(噻吩-3-基)丙烯酮(b)。 采用超快激光Z-扫描技术(脉宽180 fs,波长532 nm)测定了化合物a和b的三阶非线性光学性质。 结果表明,化合物a吸收系数β=-2.1×10^-12 m/W,折射率n₂=1.9×10^-19 m²/W,分子超极化率γ=5.37×10^-32 esu;化合物b:β=-1.2×10^-13 m/W,n₂=2.0×10^-19 m²/W,γ=4.48×10^-32 esu。 说明在飞秒激光激发下,电荷转移能够在化合物a和b分子内部快速进行,二者均具有优异的超快三阶非线性光学响应。 在B3LYP/6-311+G(d,p)理论水平下,计算了化合物a和b分子轨道能量、极化率和各基团在前线分子轨道中的占有率。 理论计算结果显示,二茂铁基团在化合物a和b前线分子轨道中占有率分别为97%和98%,对两化合物的非线性光学性能起主导作用。     

基于一维双螺旋链的锌配合物的合成与荧光性能

选择配体N,N'-双(3-吡啶)丙二酰胺(3-bpma)、1,4-对苯二乙酸(H₂pda)和硝酸锌在水热条件下,自组装制备了一个基于双螺旋链的三维超分子锌配合物[Zn(3-bpma)(pda)]_n(1),并通过红外光谱、元素分析、热重分析和X射线单晶衍射分析进行了晶体结构表征。 单晶结构分析表明标题锌配合物是正交晶系,Pna21空间群,晶胞参数a=1.62512(11) nm,b=1.15947(8) nm,c=1.19282(8) nm,α=90°,β=90°,γ=90°,V=2.2476(3) nm³,M_r=513.80,D_c=1.518 g/cm³,Z=4,F(000)=1056,R₁=0.0381,wR₂=0.0669。 金属锌离子被两种桥连配体3-bpma和pda连接形成一种一维双螺旋链状结构,相邻的链间进一步通过氢键作用拓展成为三维超分子网络结构。 标题锌配合物具有强荧光发射特性,而且其对不同的有机溶剂分子和金属离子有显著的荧光传感特性,可以作为检测硝基苯的高灵敏性荧光传感材料。 CCDC:1811967     

双核茂金属催化剂的合成、表征与应用

使用桥连配体锂盐与MCl₄络合, 合成了4个不同结构的双核茂金属化合物[μ,μ-(CH₂)₃]{[C(H)·(η⁵-C₅H₄)(η⁵-C₁₃H₈)](MCl₂)}₂[M=Zr or Ti](4, 5)和[μ,μ-(CH₂)₃]{[C(H)(η⁵-C₅H₄)(η⁵-C₉H₆)]·(MCl₂)}₂[M=Zr or Ti](6, 7), 配体和化合物都经过核磁氢谱(¹H NMR)、 碳谱(¹³C NMR)、 红外光谱(IR)及元素分析等表征, 确认了化学结构. 以甲基铝氧烷(MAO)为助催化剂, 化合物4~7为催化剂催化丙烯聚合, 考察了聚合温度、 乙烯压力、 铝钛或铝锆比对催化剂活性及聚合物分子量的影响. 结果表明, 多亚甲基桥连双核茂金属是高活性乙烯和丙烯聚合催化剂, 乙烯聚合活性最高达到7.5× 10⁶ g PE/(mol Zr·h)(化合物6), 丙烯聚合活性达 10 × 10⁵ g sPP/(mol Zr·h)(化合物4). 所得间规聚丙烯(sPP)的间规度指数(SI, r) 达到90%. 在同样条件下, 双核化合物的催化活性、 聚合物分子量M_w(> 100000)以及分子量分布(MWD>2.5)均比相应的单核化合物高(M_w<70000, MWD≤2), 表明该体系中存在较强的核效应.     

α-氨基酸及其酯化物侧链对其β-环糊精复合物稳定常数的影响

为了探索α-氨基酸及其酯化物的侧链R基团对其与环糊精非共价复合物结合强度的影响, 将一定摩尔比的β-环糊精(β-CD)分别与L型正缬氨酸(n-Val)、 亮氨酸(Leu)、 苯丙氨酸(Phe)、 天冬氨酸(Asp)、 天冬氨酸-4-苄酯(Asp-4-benzyl ester)和天冬氨酸-4-叔丁酯(Asp-4-t-butyl ester)在室温下混合, 反应平衡后采用电喷雾电离质谱进行竞争反应检测, 并以改进的质谱滴定结合曲线拟合法计算结合常数. 结果表明, 它们均可形成摩尔比为1∶1的非共价复合物. 在2组竞争反应中, 复合物的结合强度顺序分别为[β-CD∶Asp-4-benzyl ester+H]⁺>[β-CD∶Asp-4-t-butyl ester+H]⁺>[β-CD∶Asp+H]⁺以及[β-CD∶Phe+H]⁺>[β-CD∶Leu+H]⁺>[β-CD∶n-Val+H]⁺. 质谱滴定曲线拟合法测得[β-CD∶n-Val+H]⁺, [β-CD∶Asp+H]⁺, [β-CD∶Asp-4-t-butyl ester+H]⁺, [β-CD∶Asp-4-benzyl ester+H]⁺, [β-CD∶Leu+H]⁺和[β-CD∶Phe+H]⁺的稳定常数(lgK_st)分别为1.81, 2.54, 3.14, 3.26, 3.36和3.67, 结合强度依次增强. 竞争反应的定性分析结果与质谱滴定定量法测得结合强度结果的趋势一致. 由于所选用的α-氨基酸及其酯化物客体的羧基端(—COOH)和氨基端(—NH₂)均相同, 且都为亲水基团, 仅有侧链R基团不同, 因此在溶液中客体分子受疏水驱动与β-CD主体靠近并结合时, 侧链R基团的疏水力和极性2个因素起重要作用. 由于客体分子体积小, 其碳端的羧基还可与β-CD大口或小口边缘的羟基形成氢键, 使复合物更加稳定.     

(S)-(+)-1-Methyl-2-(6,7,-dimethoxy-2,3-naphthalimido)ethyl trifluoromethanesulfonate as a fluorescence chiral derivatizing reagent for carboxylic acid enantiomers in high-performance liquid chromatography

A new triflate-type fluorescence chiral derivatizing reagent, (S)-(+)-1-methyl-2-(6,7-dimethoxy-2,3-naphthalimido)ethyl trifluoromethanesulfonate, [S-(+)-MDNE-OTf], has been developed for the determination of the enantiomers of carboxylic acids. By introducing the two methoxy groups on the naphthalimido ring moiety, the red shift in the fluorescence spectrum and a high resolution in reversed-mode separation of the diastereomers of chiral carboxylic acids have been achieved. The detection limits (S/N=3) with ultraviolet and fluorescence detection are 8 fmol (λ_max=283 nm) and 4 fmol (λ_ex=283 nm, λ_em=467 nm), respectively.     

Determination of rhodamine 123 by sequential injection technique for pharmacokinetic studies in the rat placenta

The sequential injection (SIA) technique was applied in pharmacokinetic studies of the transporter-mediated passage of a model substrate, rhodamine 123 (Rho123), through the dually perfused rat term placenta. The method described was used for real-time monitoring of Rho123 concentrations in both the maternal and fetal compartments. Determination was processed by fluorescence detection (λ_ex=480 nm, λ_em580 nm); calibration curve was linear over the range 0.01–50 μmol l⁻¹ (r=0.99965), detection limit was 10 nmol l⁻¹ (3σ) and RSD2% (10 readings). Transport of Rho123 was scanned under various conditions (ATP-synthesis inhibition) and several inhibitors of P-glycoprotein transporter were tested (e.g. quinidine). The advantages of the modern SIA method—an automated analytical tool providing both fast and precise analysis—were successfully demonstrated for examination of transport profiles to investigate the effect of P-glycoprotein on the placental transfer of Rho123.     

Determination of chromophore charge states in the low pH color transition of the fluorescent protein Rtms5 via time-dependent DFT

The red fluorescent protein Rtms5^H146S displays a transition from blue (absorbance λ_max 590 nm) to yellow (absorbance λ_max 453 nm) upon titration to low pH. The pK_a of the reaction depends on the concentration of halide, offering promise for new expressible halide sensors. The protonation state involved in the low pH form of the chromophore remains, however, ambiguous. We report calculated excitation energies of different protonation states of an RFP chromophore model. These suggest that the relevant titration site is the phenoxy moiety of the chromophore, and the relevant base and conjugate acid are anionic and neutral chromophore species, respectively.     

Flow-injection on-line oxidizing fluorimetry and solid phase extraction for determination of thioridazine hydrochloride in human plasma

A simple, sensitive and specific fluorimetric method has been developed for the determination of thioridazine hydrochloride in human plasma involving solid phase extraction (SPE). In a flow-injection system, thioridazine hydrochloride is on-line oxidized into a strongly fluorescent compound with a lead dioxide solid-phase reactor and the fluorescence intensity is measured with a fluorescence detector (λ_ex = 349 nm, λ_em = 429 nm). A comparison of plasma sample pretreatment between SPE procedure and precipitation method was made and the results showed that SPE procedure was better than precipitation method. Under the optimum conditions, the fluorescence intensity is proportional to the concentration of thioridazine hydrochloride in the range from 0.015 to 2.000 μg mL⁻¹. The detection limit is 5.5 ng mL⁻¹ of thioridazine hydrochloride and the relative standard deviation is 1.06%. This method has been applied to determination of thioridazine hydrochloride in real patients plasma samples with the results compared with those obtained by HPLC method.     

Automated sequential injection fluorimetric determination and dissolution studies of Ergotamine Tartrate in pharmaceuticals

A fully automated flow system for drug-dissolution studies based on the sequential injection analysis (SIA) was described and used for monitoring dissolution profiles of Ergotamine Tartrate (ET) in pharmaceutical formulations. 50 μl of dissolution medium was taken for each measurement at a flow rate of 40 μl s⁻¹ and detected by fluorescence detector using λ_ex=236 nm (λ_em≥390 nm). The calibration curve was linear over the range 0.03–0.61 mg l⁻¹ of ET (sufficient for the dissolution tests). Equation of the calibration curve was calculated giving the following values: F=117.7 c+0.80 (n=6); r=0.9998. Detection limit was 0.01 mg l⁻¹ of ET. The R.S.D. is less than 0.54 and 0.86% (n=10) when determining 0.61 and 0.03 mg l⁻¹ of ET in standard solution, respectively. The dissolution test of Bellaspon tablets (0.3 mg of ET in 1 tablet) was programmed for 20 min, with a continuous sampling rate of 120 h⁻¹ under conditions required by BP 1993.     

Isolation and characterization of methoxylated flavones in the flowers of Primula veris by liquid chromatography and mass spectrometry

Characterization of six flavones, which were named substances G1, G2, G3, G4, G5 and G6 according to their R_F values in normal-phase thin-layer chromatography, is reported. The pure flavones were purified after maceration with methanol by normal-phase solid-phase extraction, normal-phase medium-pressure liquid chromatography, normal-phase preparative thin-layer chromatography and preparative reversed-phase high-performance liquid chromatography (RP-HPLC). The collected fractions of several isolation steps were analyzed by normal-phase (NP) and RP-HPLC. Detection and identification of the substances G was accomplished by UV detection at 213–216 nm, diode array UV detection, or fluorescence detection (λ_ex=330 nm; λ_em=440 nm). The molecular mass, the elementary composition, and the structure of the six components was determined by electron-impact high-resolution mass spectrometry (EI-HRMS). Substance G4 was identified as 3′,4′,5′-trimethoxyflavone. The substances G1–G6 were shown to be mono-, di- tri- and pentamethoxyflavones. HPLC–electrospray ionization tandem mass spectrometry (ESI-MS–MS) of the flavones was carried out employing a 150×2 mm I.D. column packed with a 3 μm/100 Å octadecylsilica stationary phase and a mobile phase comprising 1.0% acetic acid in water–acetonitrile (50:50). Comparative RP-HPLC–ESI-MS of the raw methanol extract and the isolated substances G1–G6 proved that the isolated compounds were pure and were not artifacts. Finally, RP-HPLC–ESI-MS–MS was used to identify substances G1–G6 in phytopharmaceutical drugs.     

Determination of histamine and some other amines by high-performance capillary electrophoresis with on-line mode in-capillary derivatization

We have developed a method for the determination of histamine (His), tyramine (Tyr) and cadaverine (Cad) using high-performance capillary electrophoresis with fluorescence detection and an on-line mode in-capillary derivatization with o-phthalaldehyde (OPA)/N-acetylcysteine (NAC) as derivatization reagent. HPCE separation of His, Tyr, Cad and Spermidine (Spd) was influenced by sodium dodecyl sulfate (SDS) and phosphate–borate buffer (pH 10) concentration. After optimization of the method, a 4-component amine solution containing His, Tyr, Cad and Spd could be separated and detected by using 2 mM OPA/NAC–20 mM SDS–20 mM phosphate–borate buffer (pH 10) as a run buffer at an applied voltage of 25 kV, with detection at 340 nm. Although a practical sensitivity level can be obtained by using fluorescence detection (λ_ex=340 nm, λ_em=450 nm) instead of ultraviolet–visible detection, Spd was not detected at all. The precision (relative standard deviation; n=15) of this method for within- and between-days is less than 2.9% (peak area) and 1.3% (migration time), respectively. Linearity for these analytes, except for Spd, was established over a concentration range of 0.02 to 1.00 μmol/ml and detection limits (S/N=3) range from 1 nmol/ml for His and Tyr to 5 nmol/ml for Cad. The determination of His and some amines in aging raw fish meat samples (room temperature, 48 h) was carried out using the described method with fluorescence detection.     

Spectrofluorimetric determination of levofloxacin in tablets, human urine and serum

A spectrofluorimetric method to determine levofloxacin is proposed and applied to determine the substance in tablets and spiked human urine and serum. The fluorimetric method allow the determination of 20–3000 ng ml⁻¹ of levofloxacin in aqueous solution containing acetic acid–sodium acetate buffer (pH 4) with λ_exc=292 and λ_em=494 nm, respectively. Micelle enhanced fluorescence improves the sensibility and allows levofloxacin direct measurement in spiked Human serum (5 μg ml⁻¹) and urine (420 μg ml⁻¹), in 8 mM sodium dodecyl sulphate solutions at pH 5.     

Immobilization enzyme fluorescence capillary analysis for determination of lactic acid

A new method for the determination of lactic acid based on the immobilization enzyme fluorescence capillary analysis (IE-FCA) was proposed. Lactic dehydrogenase (LDH) was immobilized on inner surface of a capillary with glutaraldehyde, and an immobilized enzyme lactate capillary bioreactor (IE-LCBR) was formed for the determination of lactic acid. After nicotinamide adenine dinucleotide (NAD⁺) is mixed with lactic acid solution, it was sucked into the IE-LCBR and was detected at λ_ex 353 nm/λ_em 466 nm. Optimized conditions are as follows: the temperature is 38 °C; the reaction time is 15 min; the concentrations of Tris buffer (pH 8.8) and NAD⁺ are 0.1 mol L⁻¹ and 4 mmol L⁻¹, respectively; the concentration of LDH used for immobilization is 15 kU L⁻¹. The concentration of lactic acid is directly proportional to the fluorescence intensity measured from 0.50 to 2.0 mmol L⁻¹; and the analytical recovery of added lactic acid was 99–105%. The minimum detection limit of the method is 0.40 mmol L⁻¹ and sensitivity of the IE-CBR is 4.6 F mmol⁻¹ L⁻¹ lactate. Its relative standard deviation (R.S.D.) is ≤2.0%. This IE-FCA method was employed for determination of lactate in milk drink.     

Spectral characterization of a novel near-infrared cyanine dye: a study of its complexation with metal ions

The spectral features of the near-infrared (NIR) dye TG-170 in different solutions and its complexation with several metal ions were investigated. The absorbance maxima of the dye are at λ=819, 805, and 791 nm in dimethyl sulfoxide (DMSO), methanol, and a buffer of pH 5.9, respectively. These values match the output of a commercially available laser diode (780 nm), thus making use of such a source practical for excitation. The emission wavelengths of the dye are at λ_em =822, 812, and 803 nm in DMSO, methanol, and the buffer, respectively. The molar absorptivity and fluorescence quantum yield increase accordingly. The addition of either an Al(III) ion or Be(II) ion resulted in fluorescence quenching of the dye. The Stern–Volmer quenching constant, K_SV, was calculated from the Stern–Volmer plot to be K_SV=3.11×10⁵ M⁻¹ for the Al(III) ion and K_SV=1.17×10⁶ M⁻¹ for the Be(II) ion. The molar ratio of the metal to the dye was established to be 1:1 for both metal ions. The stability constant, K_S, of the metal–dye complex was calculated to be 4.37×10⁴ M⁻¹ for the Al–dye complex and 1.94×10⁶ M⁻¹ for the Be–dye complex.