A study of redox properties of hydralazine hydrochloride,an antihypertensive drug

Hydralazine hydrochloride itself is a reducing agent and its redox properties like other reducing agents vary as the oxidizing agent and applied conditions vary. The redox properties of hydralazine were studied by spectrophotometric method. Formal redox potential of hydralazine was calculated and effect of pH was observed on redox properties of hydralazine.     

Time-resolved electrochemiluminescence of platinum(II) coproporphyrin

Cathodic pulse polarisation of oxide-covered aluminium electrodes can generate electrochemiluminescence (ECL) from metalloporphyrins. This is based on the tunnel emission of hot electrons into aqueous electrolyte solution, which probably results in the generation of hydrated electrons as reducing mediators. These tunnel emitted electrons allow the production of highly reactive radicals, such as sulfate radicals from peroxodisulfate ions, which can induce strong redox luminescence from various organic chemiluminophores including metalloporphyrins. The work presented here illustrates the generation of ECL from platinum(II) coproporphyrin (PtCP) and its bovine serum albumin (BSA) conjugate. This allows the detection of these molecules below nanomolar concentrations and over several orders of magnitude of concentration. The relatively long luminescence lifetime of PtCP allows discrimination from the background ECL signal using time resolved measurements, leading to higher sensitivity and the detection of PtCP-BSA indicates the potential use of metalloporphyrins as labels in ECL-based bioassays such as immunoassays and DNA-binding assays.     

Time-resolved ultraviolet laser-induced breakdown spectroscopy for organic material analysis

Ultraviolet pulses (266 nm) delivered by a quadrupled Nd:YAG laser were used to analyze organic samples with laser-induced breakdown spectroscopy (LIBS). We present characteristics of the spectra obtained from organic samples with special attentions on the emissions of organic elements, O and N, and molecular bonds CN. The choice of these atomic or molecular species is justified on one hand, by the importance of these species to specify organic or biological materials; and on the other hand by the possible interferences with ambient air when laser ablation takes place in the atmosphere. Time-resolved LIBS was used to determine the time-evolution of line intensity emitted from these species. We demonstrate different kinetic behaviors corresponding to different origins of emitters: native atomic or molecular species directly vaporized from the sample or those generated through dissociation or recombination due to interaction between laser-induced plasma and air molecules. Our results show the ability of time-resolved UV-LIBS for detection and identification of native atomic or molecular species from an organic sample.     

Time-resolved fluoroimmunoassay for ractopamine in swine tissue

This study describes the development and validation of a time-resolved fluoroimmunoassay (TR-FIA) for screening ractopamine (RAC) in swine tissue. The method is based on the direct competitive-type immunoassay using europium-labeled anti-RAC monoclonal antibody as a tracer and RAC–ovalbumin as a solid-phase antigen. When RAC was spiked at levels of 1–10 μg kg⁻¹, recoveries ranged from 88.2 to 118.5% for swine liver and muscle with coefficients of variation from 7.1 to 20.5%. The detection limit was 0.1 μg kg⁻¹. The proposed TR-FIA method was applied to the determination of RAC in an actual residue study and the applicability was confirmed by liquid chromatography–tandem mass spectrometry.     

Sensitive determination of captopril by time-resolved chemiluminescence using the stopped-flow analysis based on potassium permanganate oxidation

The chemiluminescent behaviour of captopril when reacted with a common oxidant, potassium permanganate in different acidic media is described, using the stopped-flow technique in a continuous-flow system. A 22 bit analogue-to-digital converter that acquires analogue signals at −10 and +10 V and allows the power supply to the peristaltic pump to be interrupted is used in the time-resolved chemiluminescence manifold to ensure rapid, efficient mixing of chemiluminescent reagent and sample immediately before reaching the detector; this results in high precision and detectability, particularly with fast, short-lived emissions.The optimum chemical conditions for the chemiluminescence emission were investigated. It was found that a weak CL emission was emitted during the oxidation of this drug with potassium permanganate in acidic solution. The effect of common emission enhancers such as formic acid, formaldehyde, glutaraldehyde, acetaldehyde, quinine, fluorescein, rhodamine B and rhodamine 6G was studied. The parameters selected were 4.0 mol L⁻¹ sulphuric acid, 0.25 mmol L⁻¹ permanganate and 0.75 mol L⁻¹ formaldehyde.Four quantitative parameters adjustable via software settings, two of them typically kinetic parameters, such as rate of the light-development reaction and rate of the light-decay reaction, and the other conventional parameters, such as maximum emission intensity and total emission area, were used to obtain linear calibration graphs with each measurement parameter. The detection limits ranged from 0.011 to 0.026 μg mL⁻¹ and R.S.D. values (n = 10) of 1.21-3.93 at a 0.50 μg mL⁻¹ and 2.01-3.41 at a 1.60 μg mL⁻¹ concentration levels were obtained. The method was satisfactorily applied to the determination of captopril in pharmaceutical preparations.     

时间分辨荧光免疫分析方法检测烟草中菌核净残留

建立了简便、灵敏地检测烟草中菌核净残留的时间分辨荧光免疫分析方法(TRFIA),及配套的无净化的快速前处理技术。采用镧系元素螯合物Eu-N1标记亲和纯化后的羊抗兔IgG示踪抗体。采用间接竞争TRFIA法建立了菌核净标准抑制曲线,方法的检出限I10为2.0μg/L;抑制终浓度I50为32.00μg/L;检测线性范围为4～128μg/L。考察了丙酮提取后33%,10%和1%的烟草基质对菌核净-TRFIA分析方法的影响,表明在1%烟叶基质条件下,建立的菌核净的抑制曲线的线性范围与标准抑制曲线趋于平行,确定烟草样品的前处理稀释倍数为100倍,计算得到基质影响因子(Im)为17.1。对烟叶样品中添加1,7和24mg/L的菌核净标样,连续3d的添加回收实验表明,方法的回收率为73%～128%,相对标准标准偏差(RSD)在4.3%～13.2%之间;烟草中菌核净的实际最低检出限为1mg/L。本方法可望用于烟草中菌核净残留的快速筛选检测。     

Time-resolved fluorescence spectroscopy for illuminating complex systems

Over the years, the emissive characteristics (spectral, temporal, and polarization) of fluorophores have been widely used to probe a wide variety of systems. Fluorescence lifetime and rotational reorientation time measurements, in particular, offer a means to elucidate key details about complex systems. Further, because fluorescence occurs on the nanosecond (10⁻⁹ s) timescale, competing or perturbing kinetic processes like collisional quenching, solvent relaxation, energy transfer, and rotational reorientation can affect the fluorescence and hence be quantified. Thus, a carefully chosen and “placed” fluorophore can serve as an reporter on a wide range of nanosecond or faster events. This contribution is divided into three sections. The Theory section discusses time-resolved anisotropy and intensity decay kinetics (time and frequency domains), pump–probe spectroscopy, and up-conversion. The second section describes time-correlated single photon counting (TCSPC) and multifrequency phase-modulation fluorescence instruments. The final section is divided into subsections on the use of time-resolved fluorescence: (1) to study solvation dynamics, biochemical systems, polymer photophysics, and organized media; (2) as a tool in the separation sciences, microscopy, and sensing; and (3) coupled with multiphoton excitation strategies.     

Time-resolved optical emission spectrometry of Q-switched Nd:YAG laser-induced plasmas from copper targets in air at atmospheric pressure

Q-switched Nd:YAG laser induced plasma from a copper target was studied by time-gated optical multichannel analyser. The features of the spectra such as the plasma background, the type of lines of the solid sample (singlet-doublet, doublet-singlet, doublet-doublet, quadruplet-doublet, quadruplet-quadruplet), the buffer gas, the intensity-time dependence and the line broadening of the neutral and ionic lines are described. Nitrogen, oxygen ion and metal oxide emission, self-absorption, pressure and Stark broadening is predominant at the onset of plasma formation. A time delay is required to reach the best analytical performance.     

Versatile ligational behavior of azopyrazolone derived from hydralazine

Five complexes of 3-methyl-4?-(phenylhydrazono)-1-phthalazinyl-2-pyrazolin-5-one (LH) were synthesized. The ligand and complexes were characterized using elemental analyses and various analytical techniques such as IR, UV, NMR, mass spectra, magnetic susceptibility measurements, and thermal decomposition studies such as TG/DTG. The geometries of the complexes with special emphasis on the versatile ligational behavior of LH are discussed. All five complexes have octahedral geometry. In four of the complexes [M(LH)Cl₃] where M?=?Fe(III)/Cr(III) and [M(LH)(OAc)₂H₂O] and M?=?Cu(II)/Ni(II), the ligand was neutral and tridentate. Another copper complex [CuL(OAc)(H₂O)₂] in which the ligand is tridentate, mono-anionic one was also obtained in an excess of aqueous solution. Antifungal studies of the compounds are also carried out.     

Time-resolved luminescent lateral flow assay technology

We here report a detection technology that integrates highly sensitive time-resolved luminescence technique into lateral flow assay platform to achieve excellent detection performance with low cost. We have developed very bright, surface-functionalized and mono-dispersed phosphorescent nanoparticles of long lifetime under ambient conditions. The phosphorescent nanoparticles have been used to conjugate with monoclonal antibody for C-reactive protein (CRP), an inflammatory biomarker. Lateral flow immunoassay devices have been developed using the conjugate for highly sensitive detection of CRP. The CRP assay can achieve a detection sensitivity of <0.2 ng mL⁻¹ in serum with a linear response from 0.2 to 200 ng mL⁻¹ CRP. We have also developed a low cost time-resolved luminescence reader for the lateral flow immunoassay (LFIA) devices. The reader does not use expensive band pass filter and still provide very low detection background and high detection sensitivity on solid substrates such as nitrocellulose membranes. The reader can detect less than 2.5 ng phosphorescent particles captured on a nitrocellulose membrane strip with more than three orders of magnitude linear detection dynamic range. The technology should find a number of applications, ranging from clinical diagnostics, detection of chemical and biological warfare agents, to food and environmental monitoring.     

Time-resolved fluorescence analysis of the mobile flavin cofactor in p -hydroxybenzoate hydroxylase

Conformational heterogeneity of the FAD cofactor in p-hydroxybenzoate hydroxylase (PHBH) was investigated with time-resolved polarized flavin fluorescence. For binary enzyme/substrate (analogue) complexes of wild-type PHBH and Tyr222 mutants, crystallographic studies have revealed two distinct flavin conformations; the ‘in’ conformation with the isoalloxazine ring located in the active site, and the ‘out’ conformation with the isoalloxazine ring disposed towards the protein surface. Fluorescence-lifetime analysis of these complexes revealed similar lifetime distributions for the ‘in’ and ‘out’ conformations. The reason for this is twofold. First, the active site of PHBH contains various potential fluorescence-quenching sites close to the flavin. Fluorescence analysis of uncomplexed PHBH Y222V and Y222A showed that Tyr222 is responsible for picosecond fluorescence quenching free enzyme. In addition, other potential quenching sites, including a tryptophan and two tyrosines involved in substrate binding, are located nearby. Since the shortest distance between these quenching sites and the isoalloxazine ring differs only little on average, these aromatic residues are likely to contribute to fluorescence quenching. Second, the effect of flavin conformation on the fluorescence lifetime distribution is blurred by binding of the aromatic substrates: saturation with aromatic substrates induces highly efficient fluorescence quenching. The flavin conformation is therefore only reflected in the small relative contributions of the longer lifetimes.     

Simultaneous stopped-flow determination of morphine and naloxone by time-resolved chemiluminescence

The first application of the flow analysis coupled with chemiluminescence detection and based on stopped-flow chemistry to the simultaneous determination of two components, using a two equation system, is described. The proposed method to determine simultaneously morphine and naloxone is based on the chemiluminescence oxidation of these compounds by their reaction with potassium permanganate in an acidic medium. The main feature of the system used is that the recording of the whole chemiluminescence intensity-versus-time profiles can be obtained, using the stopped-flow technique in a continuous-flow system. Then, the chemiluminescent signals obtained at two times of these profiles can be used to determine the concentration of both opiate narcotics. The effect of common emission enhancers on the chemiluminescence emission of these compounds in different acidic media, using the above-mentioned technique, was studied, in order to achieve the best conditions in which, the CL profiles of both compounds should be additive. The parameters selected were sulphuric acid 1.0 mol L⁻¹, permanganate 0.2 mmol L⁻¹ and formaldehyde 0.8 mol L⁻¹. Taken in account the different profiles of the transient CL signal obtained with each compounds, using the selected chemical conditions, two measurement times (1.4 and 4.8 s) of these responses curves were considered with the purpose to establish a simple 2 × 2 matrix calculation. Using the chemiluminiscent signals obtained at these times, a linear calibration graph was obtained for each one of the compounds between 0.01 and 1.00 mg L⁻¹ for morphine and 0.10–1.50 mg L⁻¹ for naloxone. The present chemiluminescence procedure was applied to the determination of both compounds in mixtures and was found to be satisfactory.     

Time-resolved ESI-MS Investigation on Reduction and Alkylation in Unfolding Process of Lysozyme

The kinetic procedure of the unfolding of lysozyme induced by the reduction of disulfide was monitored by the time-resolved ESI-MS with a sheath liquid assistant electrospray interface. It was found that the reduction process for the eight disulfides had a less difference in the reaction time after denatured treatment. In addition, the alkylation of the reduced free thiols was much slower than the reduction procedure. An artifact peak produced by the CID fragmentation in the mass spectra was identified and the possible mechanism of the Hofmann elimination reaction was proposed.     

时间分辨光谱技术研究亚甲基蓝与小牛胸腺DNA的相互作用

采用时间分辨光谱技术研究了亚甲蓝与小牛胸腺DNA（MB-ctDNA）重水混合体系中MB敏化单态氧（1O2）动力学过程,以此进一步探讨MB与DNA的相互作用。结果表明显示,低浓度ctDNA和高浓度ctDNA的单态氧磷光动力学曲线有着明显不同,这些差异被归结为MB与DNA间结合方式和作用机制的改变。在低浓度ctDNA条件下,MB分子和ctDNA之间形成离子型结合物,MB的吸收带出现显著的减色效应,敏化1O2产量随DNA浓度增加而急剧下降,但ctDNA与1O2没有发生明显的相互作用;而在高浓度DNA时,MB分子和ctDNA之间的相互作用方式转变为以嵌入式结合为主,激发态MB与ctDNA间的能量转移和介质的粘度效应,改变了1O2的动力学特性,大大降低了光敏剂MB敏化1O2的产量,但1O2不为ctDNA所猝灭。这些结果阐明,在MB与DNA的混合体系中,敏化单态氧损坏DNA的Ⅱ型反应不是主要的PDT作用机制。     

Development of a heterogeneous chemiluminescent flow immunoassay for DDT and related compounds

A heterogeneous chemiluminescent (CL) flow immunoassay for DDT was optimized comparing different types of immunoaffinity supports: beads, nylon coils and membranes (membranes HyBondN+). In order to characterize solid immunoaffinity supports two basic immunoassay formats were performed, using (1) enzyme-labeled secondary and (2) enzyme-labeled specific monoclonal antibodies (MAbs). In both formats, hapten DDT5 conjugated to ovalbumin immobilized on solid supports according to the appropriate immobilization procedure, enzyme label (horseradish peroxidase, HRP) and luminescent detection (luminol/H₂O₂/p-iodophenol) were used. The lowest limit of detection (LOD), 1 nM p,p-DDT, was obtained with a membrane-based flow immunoassay with HRP-labeled specific antibody. Beads and packed tubing were discarded as appropriate supports because of the difficulties encountered for reproducible packing and the occurrence of light scatterring (beads), which seriously compromised the performance and reproducibility of the flow immunoassay.     

A signal-on electrogenerated chemiluminescent biosensor for lead ion based on DNAzyme

A highly reproducible and sensitive signal-on electrogenerated chemiluminescence (ECL) biosensor based on the DNAzyme for the determination of lead ion was developed. The ECL biosensor was fabricated by covalently coupling 5′-amino-DNAzyme-tagged with ruthenium bis (2,2′-bipyridine) (2,2′-bipyridine-4,4′-dicarboxylic acid)-ethylenediamine (Ru1-17E′) onto the surface of graphite electrode modified with 4-aminobenzoic acid, and then a DNA substrate with a ribonucleotide adenosine hybridized with Ru1-17E′ on the electrode. Upon binding of Pb²⁺ to the Ru1-17E′ to form a complex which catalyzed the cleavage of the DNA substrate, the double-stranded DNA was dissociated and thus led to a high ECL signal. The signal linearly increases with the concentration of Pb²⁺ in the range from 5.0 to 80 pM with a detection limit of 1.4 pM and a relative standard derivation of 2.3%. This work demonstrates that using DNAzyme tagged with ruthenium complex as an ECL probe and covalently coupling method for the fabrication of the ECL biosensor with high sensitivity, good stability and significant regeneration ability is promising approach.     

流动注射化学发光检测盐酸异丙嗪

在碱性介质中,盐酸异丙嗪对luminol-KMnO4发光体系有显著的增强作用.基于此增强作用,建立了一种FI-CL检测盐酸异丙嗪的新方法.在最优化的实验条件下,盐酸异丙嗪的ΔICL强度与其浓度在7.0×10-9~9.0×10-7 mol/L浓度范围内有较好的线性关系.线性方程为ΔICL=35.19+1.19×10-10 c,相关系数r=0.998 4,检出限为4.9×10-9 mol/L.对7.0×10-9 mol/L的盐酸氯丙嗪标准溶液进行11次平行测定,其RSD为2.4%.盐酸异丙嗪加标回收率在89.1%~96.1%之间.     

Time-resolved enzymatic determination of glucose using a fluorescent europium probe for hydrogen peroxide

An enzymatic assay for glucose based on the use of the fluorescent probe for hydrogen peroxide, europium(III) tetracycline (EuTc), is described. The weakly fluorescent EuTc and enzymatically generated H₂O₂ form a strongly fluorescent complex (EuTc–H₂O₂) whose fluorescence decay profile is significantly different. Since the decay time of EuTc–H₂O₂ is in the microseconds time domain, fluorescence can be detected in the time-resolved mode, thus enabling substantial reduction of background fluorescence. The scheme represents the first H₂O₂-based time-resolved fluorescence assay for glucose not requiring the presence of a peroxidase. The time-resolved assay (with a delay time of 60 s and using endpoint detection) enables glucose to be determined at levels as low as 2.2 mol L^–1, with a dynamic range of 2.2–100 mol L^–1. The method also was adapted to a kinetic assay in order to cover higher glucose levels (mmol L^–1 range). The latter was validated by analyzing spiked serum samples and gave a good linear relationship for glucose levels from 2.5 to 55.5 mmol L^–1. Noteworthy features of the assay include easy accessibility of the probe, large Stokes shift, a line-like fluorescence peaking at 616 nm, stability towards oxygen, a working pH of approximately 7, and its suitability for both kinetic and endpoint determination.     

Fiberoptic biosensors based on chemiluminescent reactions

The chemiluminescence of luminol in the presence of H₂O₂ has been exploited to develop fiberoptic biosensors associated with flow injection analysis systems. A chlorophenol sensor was developed based on the ability of certain halophenols to enhance the peroxidase-catalyzed luminol chemiluminescence. Horseradish peroxidase immobilized on a collagen membrane was used. Ten chlorophenols have been tested with this chemiluminescent-based sensor. The lower detection limit was obtained with 4-chloro-3-methylphenol and was equal to 0.01 μM. Electrochemiluminescent-based fiberoptic biosensors for glucose and lactate were also developed using glucose oxidase or lactate oxidase immobilized on polyamide membranes. In the presence of oxidase-generated H₂O₂, the light emission was triggered electrochemically by means of a glassy carbon electrode polarized at +425 mV vs a platinum pseudo-reference electrode. The detection limits for glucose and lactate were 150 and 60 pmol, respectively, and the dynamic ranges were linear from 150 pmol to 600 nmol and from 60 pmol to 60 nmol, respectively.