FT-Raman,FT-infrared and NIR spectroscopic characterization of oxygen-delignified kraft pulp treated with hydrogen peroxide under acidic and alkaline conditions

The effects of bleaching treatment of oxygen-delignified softwood kraft pulp with hydrogen peroxide under acidic and alkaline conditions were studied using standard technological techniques and spectroscopic analytical methods: near-infrared (NIR), Fourier-transform infrared (FTIR) and Fourier-transform (FT) Raman spectroscopies. Among the three tested spectroscopic techniques, NIR analysis appeared to be the most appropriate in terms of possible technological applications. The use of NIR spectroscopy combined with multivariate data analysis allowed to create models for pulp bleaching monitoring based on CIE L*a*b* measurements. Near-infrared and FTIR spectroscopic studies allowed differentiating between the effects of the acidic and alkaline peroxide bleaching stages, but failed in relation to the delignification process. The most representative bands in the FTIR and FT-Raman spectra in terms of delignification and chromophore removal exhibited no correlation with standard technological measurement results.     

酶催化动力学光度法测定H2O2

H2O2能够氧化偶氮染料刚果红使之褪色,而模拟酶—血红蛋白对其具有催化作用。据此建立了一种以刚果红为指示剂的H2O2-刚果红-血红蛋白酶催化反应体系测定痕量H2O2的新方法。确定了反应的最佳条件,体系的酸度为pH10.7的NH3-NH4Cl缓冲溶液,最大吸收波长为497 nm。该法的线性范围为8.0×10^-8-8.0×10^-5mol/L,检出限为1.97×10^-9mol/L,表观摩尔吸光系数为4.6×10^4L.mol-1.cm^-1。该方法可用于雨水及消毒水中H2O2的测定。     

过氧化氢氧化灿烂甲酚蓝动力学光度法测定痕量铝

基于pH3.6的乙酸 乙酸钠缓冲介质中Al3 对过氧化氢氧化灿烂甲酚蓝(BCB)褪色反应的催化作用,提出了测定痕量铝的新的催化动力学光度法。研究了该法的适宜反应条件,方法的线性范围为0～100ng mL,检出限为0.9ng mL。方法已用于样品中痕量铝的测定。     

Rapid determination of hydrogen peroxide in whitening patches for teeth using a new portable near-infrared spectrometer

A nondestructive determination method of hydrogen peroxide in whitening patches for teeth was developed by using a new portable near-infrared (NIR) spectrometer. Development of the portable NIR spectrometer was based on microchip technologies with photodiode arrays. By using the portable NIR spectrometer, the new determination method is very rapid; it requires less than 1 s. The conventional method for the determination of hydrogen peroxide, redox titration, requires about 2 h of analysis, including the sample extraction time from a sample matrix. The conventional method also uses hazardous and harmful solvents and, furthermore, its samples cannot be used after titration. To find the peak due to the O–H bond vibration of hydrogen peroxide under the existence of water which shows huge absorption O–H absorption around 1450 nm, the NIR spectra of a hydrogen peroxide aqueous solution were investigated. A clear variation of absorption based on the concentration of the hydrogen peroxide due to the O–H bond vibration was found in the standard deviation plot around 1400 nm. In this study, two kinds of whitening patch products, A and B, were used for samples. A partial least squares (PLS) regression was used for calibration and validation in the 1100 to 1720 nm spectral range. For validation results, the standard error of prediction (SEP) was 0.38% for Patch A and 0.37% for Patch B. This study shows the feasibility of using the portable NIR spectrometer with photodiode arrays for the rapid and safe determination of hydrogen peroxide in whitening patches.     

Spectrophotometric determination of hydrogen peroxide in rainwater

Hydrogen peroxide in rainwater has been determined from the measurement of absorption at 432 nm after the formation of the stable oxo-peroxo-pyridine-2,6-dicarboxylatovanadate(V) complex (OPDV) in acid media. Determinations were in good agreement with those using a modified p-hydroxyphenylacetic acid (PHPA) emission method. The linear range for the OPDV method is from 0.05 to 50 ppm H₂O₂, and the limit of detection under the analytical conditions employed was 5.8 nmol H₂O₂ for a 20 cm³ rainwater sample. The volume weighted mean H₂O₂ concentration in rainwater collected at roof-top level in central Kowloon was 15.9 μM (N=10), and the ratio of non-sea salt sulphate and H₂O₂ concentrations was significantly correlated with pH. The OPDV absorption method was also employed for the determination of ambient gaseous H₂O₂, and liquid-nitrogen cold-trap collection gave results about 30% lower than impinger sampling, where artifact H₂O₂ formation occurred.     

Pretreatment of wastepaper and pulp mill sludge by aqueous ammonia and hydrogen peroxide

Pretreatment of two different softwood-based lignocellulosic wastes (newsprint and Kraft pulp mill sludge) was investigated. Pretreatment was done by aqueous ammonia and hydrogen peroxide (H₂O₂), two delignifying reagents that are environmentally benign. Three different treatment schemes were employed: aqueous ammonia alone (ammonia recycled percolation [ARP]), mixed stream of aqueous ammonia and H₂O₂ and successive treatment with H₂O₂ and aqueous ammonia. In all cases there was a substantial degree of delignification ranging from 30 to 50%. About half of the hemicellulose sugars were dissolved into the process effluent. Retention of cellulose after pretreatment varied from 85 to 100% for newspaper feedstock and from 77 to 85% for the pulp mill sludge. After treatment with aqueous ammonia alone (ARP), the digestibility of newspaper and the pulp mill sludge was improved only by 5% (from 40 to 45% for the former and from 68 to 73% for the latter), despite a substantial degree of delignification occurring after the ARP process. The lign in content thus did not correlate with the digestibility for these substrates. Simultaneous treatment with H₂O₂ and aqueous ammonia did not bring about any significant improvement in the digestibility over that of the ARP. A succcessive treatment by H₂O₂ and ARP showed the most promise because it improved the digestibility of the newspaper from 41 to 75%, a level comparable to that of α-cellulose.     

A chemiluminescence sensor for the determination of hydrogen peroxide

A chemiluminescence one-shot sensor for hydrogen peroxide is described. It is prepared by immobilization of cobalt chloride and sodium lauryl sulphate in hydroxyethyl cellulose matrix cast on a microscope cover glass. Luminol, sodium phosphate and the sample are mixed before use and applied on the membrane by a micropipette. The calibration graph is linear in the range 20-1600 μg/L, and the detection limit of the method (3σ) is 9 μg/L. A relative standard deviation of 4.5% was obtained for 100 μg/L H₂O₂ (n = 11). The sensor has been applied successfully to the determination of hydrogen peroxide in rainwater.     

Characterization of the supermolecular structure of cellulose in wood pulp fibres

The hierarchic organization of cellulose fibrils (microfibrils) was investigated in holocellulose, sulphite pulp and kraft pulp using TEM, XRD, ED and FTIR. There were remarkable differences in both the fibril structure and fibril aggregation between the samples. TEM observations revealed more intimately associated fibrils in the kraft pulp compared to the sulphite pulp and the holocellulose, results in agreement with previous CP/MAS ¹³C-NMR data [Hult E.-L. et al. (2002) Holzforschung 56: 231–234]. Furthermore, the cellulose crystallinity was higher in the kraft pulp sample. With respect to the cellulose I and I allomorphs, these samples were controversial when different analytical techniques were applied. Due to the small fibril size and the low degree of order of cellulose in these samples, the concept of crystalline triclinic and monoclinic components as determined by diffraction analysis may not be adequate. Instead the fibril can be regarded to have different degrees of lateral order (including paracrystalline ordering) that can be reoriented to I type conformation and packing upon pulping.     

Efficient total halogen-free photochemical bleaching of kraft pulps using alkaline hydrogen peroxide

Total halogen-free bleaching of kraft pulps was conducted by an oxidative photochemical process at room temperature using alkaline hydrogen peroxide. Selection of an appropriate wavelength of light was crucial for effective bleaching and avoiding degradation of cellulose. The wavelength of the light has to be selected so that the light is absorbed only by the colored compounds in the pulps and not by the bleaching reagents or the pulp itself. When a long-wavelength black-light fluorescent lamp was used in combination with aqueous hydrogen peroxide solution at pH 11, the bleaching efficiency for hardwood and softwood kraft pulps reached the same level as that obtained by conventional two-stage elemental chlorine-free processes.     

Mediated amperometric enzyme electrode incorporating peroxidase for the determination of hydrogen peroxide in organic solvents

An amperometric enzyme electrode incorporating horseradish peroxidase is described for the determination of hydrogen peroxide in organic solvents. The enzyme was co-adsorbed with an electron mediator, potassium hexacyanoferrate(II), on the surface of a graphite foil electrode, making reagentless measurement possible. The electrochemical reduction of the enzymatically oxidized mediator was utilized as the analytical signal. Studies in different solvent systems revealed that the electrode could be operated in dioxane, chloroform and chlorobenzene, the last two providing approximately double the sensitivity of the former. The presence of a small amount of aqueous buffer was essential for sensor activity. During 2 weeks of intermittent use, the sensitivity of the electrode decreased to 40% of its initial value. At least 50 assays could be performed with a single sensor.     

Biosensor for determination of hydrogen peroxide based on catalase activity of human erythrocytes

A hydrogen peroxide biosensor based on human erythrocytes is described. Erythrocytes are retained on the surface of an oxygen electrode by a semipermeable membrane. The response is based on the catalase activity of the erythrocytes. The sensitivity of 10^?4 mol 1^?1 and linearity from 1.5×10^?4 to 5×10^?3 mol^?1 are comparable to those of analogous enzyme biosensors for hydrogen peroxide determination. The greatest advantages of this biosensor are its easy preparation and a lifetime of 2 months together with good reproducibility (relative standard deviation <5%) and selectivity; only ascorbic acid appeared to interfere with the measurements.     

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.     

N,N-diethylaniline as hydrogen donor for determination of hydrogen peroxide catalyzed by metalloporphyrins as enzyme mimetic of peroxidase

Various metalloporphyrins have been used as a catalyst instead of the peroxidase for the determination of hydrogen peroxide by formation of a dye from N,N-diethylaniline (DBA) and 4-aminoantipyrine. The difference of relative catalytic activity was investigated between enzyme and enzyme mimetics. FeT(4-TAP)P [5, 10, 15, 20-tetrakis (4-trimethyl-ammoniumphenyl)-21H, 23H-porphine] was shown as the best enzyme mimetic for horseradish peroxidase (HRP) among metalloporphyrins tested. 0 to 7.0 × 10^–5 mol/L hydrogen peroxide was determined with good accuracy and reproducibility, and giving recovery of 99.7–100.7%. DEA was certified as a sensitive color reagent in enzyme mimetic assay of hydrogen peroxide, with the apparent molar absorptivity for hydrogen peroxide was 1.37 × 10⁴ L/mol·cm.     

极谱催化波法测定土霉素

H2 O2 存在时 ,产生土霉素的极谱催化波 ,该催化波的灵敏度比相应土霉素的还原波高 8倍 ,据此拟定了测定土霉素的新方法。在 0 .1 0mol LKH2 PO4 Na2 HPO4(pH 7.4± 0 .2 ) - 1 .6× 1 0 -3 mol LH2 O2 底液中 ,催化波峰电流与土霉素浓度在 5 .0× 1 0 -7～ 9.0× 1 0 -6mol L范围内呈线性关系 (n =1 0 ,r=0 9996)。检出限为 1 .0× 1 0 -7mol L。     

Catalytic decomposition of hydrogen peroxide by a flow-through self-regulating platinum black heater

A flow-through reactor where a fine platinized platinum wire (Pt black wire) runs through the entire length of the PTFE tube was fabricated for the rapid decomposition of hydrogen peroxide (H₂O₂) at concentrations up to 1 M. Since the Pt black wire is directly electrically heated and the exterior of the tubular reactor is well insulated, the energy efficiency of this heater reactor is excellent. The temperature coefficient of resistance of the wire is significant (3280±40 ppm/°C). This provides a means to ascertain the mean temperature by measuring the resistance of the wire. The concentration of residual H₂O₂ was determined by the hematin-catalyzed oxidation of nonfluorescent thiamine to fluorescent thiochrome by H₂O₂. Essentially, quantitative (99.997%) decomposition of 1 M H₂O₂ could be achieved at a mean reactor temperature of 108 °C from a neutral aqueous solution with a mean residence time of ∼270 s.     

Application of Fenton reaction for nanomolar determination of hydrogen peroxide in seawater

A simple and sensitive method for the determination of nanomolar levels of hydrogen peroxide (H₂O₂) in seawater has been developed and validated. This method is based on the reduction of H₂O₂ by ferrous iron in acid solution to yield hydroxyl radical (OH) which reacts with benzene to produce phenol. Phenol is separated from the reaction mixture by reversed phase high performance liquid chromatography and its fluorescence intensity signals were measured at excitation and emission of 270 and 298 nm, respectively. Under optimum conditions, the calibration curve exhibited linearity in the range of (0-50) × 10³ nmol L⁻¹ H₂O₂. The relative standard deviations for five replicate measurements of 500 and 50 nmol L⁻¹ H₂O₂ are 1.9 and 2.4%, respectively. The detection limit for H₂O₂, defined as three times the standard deviation of the lowest standard solution (5 nmol L⁻¹ H₂O₂) in seawater is 4 nmol L⁻¹. Interference of nitrite ion (NO₂⁻) on the fluorescence intensity of phenol was also investigated. The result indicated that the addition of 10 μmol L⁻¹ NO₂⁻ to seawater samples showed no significant interference, although, the addition of 50 μmol L⁻¹ NO₂⁻ to the seawater samples decreases the fluorescence intensity signals of phenol by almost 40%. Intercomparison of this method with well-accepted (p-hydroxyphenyl) acetic acid (POHPAA)-FIA method shows excellent agreement. The proposed method has been applied on-board analysis of H₂O₂ in Seto Inland seawater samples.     

Use of hydrogen peroxide to achieve interference-free stripping voltammetric determination of copper at the bismuth-film electrode

In this work, a new approach is presented to allow interference-free determination of Cu (II) by stripping voltammetry using the bismuth-film electrode. The addition of hydrogen peroxide to the electroanalytical cell has promoted complete resolution between re-dissolution peaks of Bi (III) and Cu (II). The absence of interference could be evaluated by the correlation coefficient (r > 0.99) between Cu (II) concentration and its shifted current peak (at +212 mV) while achieving a slightly fluctuation of the bismuth current peak at −180 mV. Studies were performed aiming towards the optimum conditions for trace determination of Cu (II) using hydrogen peroxide. The methodology was applied to a real sample (sugarcane spirits) and the results were compared to those from graphite furnace atomic absorption spectrometry. The analytical parameters of merit and the results of the analysis indicated that the analytical methodology could be readily used for trace determination of Cu (II).     

A peroxidase-tetrathiafulvalene biosensor based on self-assembled monolayer modified Au electrodes for the flow-injection determination of hydrogen peroxide

The construction and performance under flow-injection conditions of an integrated amperometric biosensor for hydrogen peroxide is reported. The design of the bioelectrode is based on a mercaptopropionic acid (MPA) self-assembled monolayer (SAM) modified gold disk electrode on which horseradish peroxidase (HRP, 24.3 U) was immobilized by cross-linking with glutaraldehyde together with the mediator tetrathiafulvalene (TTF, 1 μmol), which was entrapped in the three-dimensional aggregate formed.

The amperometric biosensor allows the obtention of reproducible flow injection amperometric responses at an applied potential of 0.00 V in 0.05 mol L⁻¹ phosphate buffer, pH 7.0 (flow rate: 1.40 mL min⁻¹, injection volume: 150 μL), with a range of linearity for hydrogen peroxide within the 2.0 × 10⁻⁷–1.0 × 10⁻⁴ mol L⁻¹ concentration range (slope: (2.33 ± 0.02) × 10⁻² A mol⁻¹ L, r = 0.999). A detection limit of 6.9 × 10⁻⁸ mol L⁻¹ was obtained together with a R.S.D. (n = 50) of 2.7% for a hydrogen peroxide concentration level of 5.0 × 10⁻⁵ mol L⁻¹. The immobilization method showed a good reproducibility with a R.S.D. of 5.3% for five different electrodes. Moreover, the useful lifetime of one single biosensor was estimated in 13 days.

The SAM-based biosensor was applied for the determination of hydrogen peroxide in rainwater and in a hair dye. The results obtained were validated by comparison with those obtained with a spectrophotometric reference method. In addition, the recovery of hydrogen peroxide in sterilised milk was tested.     

Oxidation of thiocyanate by hydrogen peroxide - a reaction kinetic study by capillary electrophoresis

The oxidation reaction kinetics of thiocyanate by excess hydrogen peroxide has been studied by using capillary electrophoresis. The paper illustrates for the first time the use of capillary electrophoresis in studying reaction kinetics and provides a non-laborious way to determine the rate law and the rate constant for the above reaction in the pH range 6–8. Standard solutions of thiocyanate were mixed with buffer solutions of different pHs (6–8) and the reactions were initiated by adding appropriate volumes of hydrogen peroxide in capillary electrophoresis vials. Each reaction mixture was sampled at regular time intervals using an automatic injection programme to follow the progress of the reaction and identify the reaction products. The peak areas, representing the products, were integrated and their concentrations were quantified using calibration plots. The concentration profiles obtained from a series of experiments at a particular pH were then used to determine the rate law and the rate constant for the reaction. Furthermore, the rate of decomposition of hypothiocyanite formed during the reaction is determined for the first time. The rate law is zero order with respect to hypothiocyanite and first order with respect to hydrogen peroxide. The results indicate that the rate law for the oxidation reaction is zero order with respect to thiocyanate and first order with respect to hydrogen peroxide. The rate constant for the reaction at 25°C and at zero ionic strength is 3.6(±0.2)×10(⁻⁴) min⁻¹.     

Hydroperoxidation of alkanes with hydrogen peroxide catalyzed by aluminium nitrate in acetonitrile

The first example of alkane oxygenation with hydrogen peroxide catalyzed by a non-transition metal derivative (aluminium) is reported. Heating (70 °C) a solution of an alkane, RH, hydrogen peroxide (70% aqueous) and a catalytic amount of Al(NO₃)₃·9H₂O in air for a few hours afforded the corresponding alkyl hydroperoxide, ROOH. With cyclooctane, the hydroperoxide yield attained 31% and the maximum turnover number was 150. It is proposed on the basis of measurements of the selectivity parameters for the oxidation of linear and branched alkanes and a kinetic study that the oxidation occurs with the participation of hydroxyl radicals.