铜离子对烟草多酚氧化酶变性和复性影响的热力学研究(英)

在有无5 mmol·L^-1 CuSO₄存在的两种情况下，运用荧光光谱研究了烟草多酚氧化酶在盐酸胍诱导下的变性和复性平衡。烟草多酚氧化酶在6.0 mol·L^-1盐酸胍变性30 min(25 ℃)即完全失活。荧光光谱结果表明：铜离子能够提高烟草多酚氧化酶的结构稳定性和抗盐酸胍变性的能力，进而影响烟草多酚氧化酶在盐酸胍诱导下的变性和复性过程。没有外源铜存在的情况下，盐酸胍诱导的烟草多酚氧化酶变性和复性是一个可逆的二态过程；在5 mmol·L^-1 CuSO₄存在的条件下，由于结合了Cu²⁺的酶的中间态稳定性增加，显示特征荧光，结果显示，外源铜存在时，盐酸胍诱导的烟草多酚氧化酶变性和复性是一个可逆的三态过程。根据相应模型，进行了热力学计算。上述实验结果得到酶活性测定的进一步证实，在6 mol·L^-1盐酸胍中放置5，10，15，20，25，30 min，烟草多酚氧化酶的剩余活性分别为18.7%，11.7%，8.9%，6.6%，3.6%，0.06%，但在5 mmol·L^-1 CuSO₄存在的条件下，剩余活性则分别为60.3%，44.6%，42.5%，40.2%，25.6%，25.3%。     

柱前衍生高效液相色谱法测定烟草中阿维菌素残留

建立了烟草中阿维菌素残留量的柱前衍生高效液相色谱测定方法。烟草样品经乙腈提取,碱性氧化铝固相萃取柱净化,以三氟乙酸酐(TFAA)-N-甲基咪唑(NMIM)-乙腈(ACN)进行柱前荧光衍生化,用高效液相色谱-荧光检测器检测。结果表明,该方法对烟草中阿维菌素残留量的最低检测浓度为0.001mg/kg,添加回收率在89.37%～102.84%之间,相对标准偏差为3.02%～4.05%(n=5)。     

一种基于分子信标荧光探针快速检测烟草花叶病毒的新方法

研究了一种利用新型荧光探针——分子信标进行植物病毒检测的方法，可以不要求对病毒RNA进行严格的分离和纯化，就能快捷地得到检测结果。此方法被用于烟草花叶病毒(tobacco mosaic virus，TMV)基因组RNA的检测，为植物病毒分子生物学的研究提供了新的手段。     

水蒸气蒸馏返滴定法测定烟草及其制品中总挥发有机酸

烟草中总挥发酸含量与烟草质量密切相关，它对烟草的口味、刺激性和香气都有重要影响，烟草中挥发有机酸测定具有重要意义。总挥发酸的测定一般先在磷酸介质中水蒸气蒸馏分离，然后采用酚酞作指示剂氢氧化钠滴定。传统的水蒸气蒸馏装置蒸馏总挥发酸耗时长，精密度较差；挥发酸多数     

柱后衍生-高效液相色谱法测定烟草中游离氨基酸

建立了柱后衍生-高效液相色谱法分离检测烟草中19种游离氨基酸的方法。样品经0.005 mol/L的盐酸超声提取,高效锂阳离子交换柱分离后,采用OPA柱后衍生,荧光检测器检测。各氨基酸在样品含量范围内呈良好的线性关系,相关系数(R2)均大于0.999,在烤烟中的加标回收率为87.73%～100.02%,相对标准偏差在2.7%～6.0%之间,检出限0.13～2.00μmol/L。方法可用于烟草中游离氨基酸的分析。     

第12届全反射X射线荧光分析以及相关方法会议(Ⅱ)

会议交流论文共33篇, 现分述如下: (1) 墨西哥T Martinez, Teothuacan城太阳金字塔下洞穴中渗入的水的物质应用全反射X射线荧光谱与其他技术测定; (2) 墨西哥T Martinez, 应用全反射X射线荧光谱技术于烟草试样中痕量元素的测定;     

微波辐照同时分离烟草中亚硝胺和氮氧化合物

利用微波辐照建立了一种同时分离烟草中挥发性亚硝胺和氮氧化物的方法，能在3min内收集烟草和烟草制品中的亚硝胺和氮氧化物；本文确定了最佳实验条件。     

固相萃取光度法测定烟草中的挥发酚

研究了用Waters Sep-Park-C18固相萃取小柱萃取测定烟草样品中的挥发酚的方法。用自动水蒸汽蒸馏仪蒸馏出烟草样品中的挥发酚，4-氨基安替比林显色，显色产物可用Waters Sep-Park-C18固相萃取小柱萃取，以乙醇洗脱后用分光光度法测定，该方法可用于烟草样品中挥发酚的测定。     

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。     

同步检测烟草丛顶病毒和烟草扭脉病毒的方法

本发明提供一种同步检测烟草丛顶病毒和烟草扭脉病毒的方法，属植物保护领域。根据烟草丛顶病毒和烟草扭脉病毒核苷酸序列分别设计两对特异性引物TB2F／TB2R（检测烟草丛顶病毒）及TVCPF／TVCPR（检测烟草扭脉病毒）。提取植株组织的总RNA后，采用双重RT—PCR的方法，同步检测烟草丛顶病毒和烟草扭脉病毒。该发明能有效克服指示植物法、电镜技术、酶联免疫技术以及总核酸提取法和传统RT—PCR方法的缺点，只用相当于一次普通RT—PCR的时间和试剂，就可以方便、特异、灵敏的同步检测烟草丛顶病毒和烟草扭脉病毒。     

Ultrasonic extraction followed by a novel filtration and clean-up device for screening of some polyphenols in tobaccos

A simple and efficient HPLC method using a diode array detector (DAD) was developed for simultaneous determination of six polyphenols in tobaccos. Ultrasonic extraction was employed at 25 degrees C to extract the polyphenols present in tobaccos into anhydrous methanol. A novel filtration device linked to a clean-up cartridge was designed for simultaneous extract filtration and clean-up. Optimized HPLC-DAD analysis, with multi-wavelength detection, was used for determination of the polyphenols. Because the content of some of the polyphenols is too low to be quantified directly, a concentration step was necessary. Anhydrous methanol was employed for extraction of the polyphenols because of its high extraction efficiency and its low boiling point in the concentration step. Using the proposed method, six polyphenols were quantified in tobaccos (Nicotina tobaccum L.).     

Comparison of methods for extraction of tobacco alkaloids

Ultrasound and microwave techniques were used to extract tobacco alkaloids, and response surface methodology was used to optimize extraction conditions. Ultrasonic technique factors were temperature, 30-85 degrees C; time, 3-45 min; solvent volume, 8-80 mL. Microwave extraction factors were pressure, 15-75 psi; time, 3-40 min; power, 30-90% of the maximum magnetron power of 650 W. Soxhlet and solvent AOAC-modified extraction methods were also applied after some improvements. Nicotine, nornicotine, anabasine, and anatabine were quantified by gas chromatography. A steam distillation International Standards Organization method for total alkaloid evaluation was used as reference. The results obtained by the different methods were compared using a least squares deviation test. The ultrasonic and the proposed modified-AOAC extraction method were the more convenient with regard to practicability and precision. The relative deviations (n = 5) were as follows: For the ultrasonic method in low-level alkaloid tobaccos, 0.7% nicotine and 1.4-14% minor alkaloids; in high-level alkaloid tobaccos, 2.4% nicotine and 4.5-5.1% minor alkaloids. For the modified AOAC method in low-level alkaloid tobaccos, 0.9% nicotine and 2.4-11.6% minor alkaloids; and in high-level alkaloid tobaccos, 1.7% nicotine and 2.0-2.4% minor alkaloids.     

Determination of sugars and alditols in tobacco with high performance anion-exchange chromatography

Sugars, alditols, and alcohols in tobacco products were quantified utilizing a method of high-performance anion-exchange chromatography-pulsed amperometric detection (HPAEC-PAD). The optimized analytical method can be used to classify different tobaccos and control the quality of tobaccos. To substantiate the applicability of the method, the analysis of 27 tobacco samples with satisfactory linearity, repeatability, and accuracy had been demonstrated. Compared with some other analytical methods for tobacco, the HPAEC-PAD method provided a simple and powerful tool for the analysis of not only sugars but also alcohols in tobacco extracts.     

Analysis of free and bound volatiles by gas chromatography and gas chromatography-mass spectrometry in uncased and cased tobaccos

The free and bound volatiles of tobaccos were analyzed by capillary GC and GC-MS. Bound volatiles were isolated by dichloromethane extraction followed by stream distillation continuous extraction (SDE) at pH 2.5 acid hydrolysis. The bound aromatic compounds were hydrolyzed by acid at pH 2.5, and the bound volatiles were liberated and extracted into dichloromethane by SDE simultaneously. In total, 23 volatiles were identified, with neophytadiene, 2-ethyl hexanol, damascenone, benzene ethanol, palmitic acid, stearic acid, linoleic acid, farnesyl acetone, 3-oxo-ionol, and megastigmatrienone being the major components. They consisted mainly of compounds exhibiting aromatic characteristics. The quality and quantity of free and bound volatiles exhibited different distributions in uncased or cased tobaccos. The volatiles existed in higher amounts in bound form than in free form. Compared with uncased tobaccos, free form volatiles showed a decrease after the casing process, while bound volatiles showed an increase.     

Water-soluble fluorescent boronic acid compounds for saccharide sensing: substituent effects on their fluorescence properties

Four new naphthalene-based boronic acid compounds (1-4) were synthesized. The effect of various carbohydrates on their fluorescence properties has been studied in aqueous phosphate buffer at pH 7.4. Different substitutions on the aniline group of the naphthalene ring resulted in significant differences in fluorescence properties for these four compounds. Compound 1 shows ratiometric fluorescence changes upon addition of a sugar. Compounds 2 and 3 do not show ratiometric fluorescence changes but show very large fluorescence intensity changes (about 70-fold fluorescence intensity increase). In addition to the quantifiable fluorescence property changes upon sugar addition, the fluorescence color changes of 1-3 are also visible to the naked eye. However, amidation of the aniline nitrogen atom significantly diminishes the fluorescence intensity of compound 4. The crystal structure of one boronic acid provided some insight into the structural features that are important for the fluorescence properties of these compounds.     

Comparison of the Solution Luminescence Properties and Solid-Matrix Luminescence Properties of 2-Amino-1-Methyl-6-Phenylimidazo[4,5-B]Pyridine

Abstract

The solution fluorescence properties of 2-amino-1-methyl-6-phenylimidazo[4,5-b]pyridine (PhIP) were compared with the solid-matrix luminescence properties of PhIP. The fluorescence properties were obtained in ethanol and several binary solutions of ethanol:water. An ethanol solution of PhIP gave a very strong fluorescence signal and the ethanol:water solutions only showed a small increase in the fluorescence signal. Acidic solutions of PhIP in ethanol:water (7:3) showed a major decrease in fluorescence intensity with at HCl of 10^?4 M and greater, but NaOH solutions of PhIP did not affect the fluorescence intensity to any great extent. Both acidic and basic solutions gave fluorescence emission spectra that were shifted to longer wavelengths. Solid-matrix room-temperature fluorescence (SMRTF) and solid-matrix room-temperature phosphorescence (SMRTP) were readily obtained on filter paper. SMRTP showed some distinct advantages over SMRTF and gave a limit of detection of 0.2 ng on filter paper. Several aspects of both solution luminescence and solid-matrix luminescence of PhIP are discussed.     

Simultaneous multielement determination of chewing and snuff tobaccos used in India by INAA

Trace elements present in Indian cigarette tobacco and cigarette smoke have been reported earlier. This paper presents trace element concentrations in chewing and snuff tobaccos determined by Instrumental Neutron Activation Analysis. The levels of Br, Co, Cr, Fe, Mn, Zn, etc., present in different brands of chewing and snuff tobaccos are compared in two types of tobacco as well as with similar data from other countries.     

Nonlinear decrease of background fluorescence in polymer thin-films - a survey of materials and how they can complicate fluorescence detection in microTAS

Polymers and plastics are receiving increased attention as materials for microfluidics and microTAS applications. Given the ubiquity of fluorescence detection techniques in micro-analytical systems, the fluorescence properties of polymers and plastics should not be overlooked. We survey some commonly available polymer thin-films for their fluorescence behaviour under standardized conditions to determine which materials are most suitable for high-sensitivity fluorescence detection lab chips. The initial fluorescence intensities of some of the materials surveyed were significantly higher than glass and fused silica controls, and decreased over the three hour period with complex kinetics. We then discuss how this has confounded fluorescence detection in our analytical context, and possible mechanisms for the decrease.     

Fluorescence response of hypocrellin B to the environmental changes in a mimic biological membrane--liposome

Liposome is well known as not only a drug-delivery system but also a simple model for biological membranes. It was reported that fluorescence properties of hypocrellins were changeable over some extreme pH values. In the current work, the effects of the microenvironments on the fluorescence properties of HB in liposome, including approximately physiological range of pH values pH = 6.0-8.0, concentration of cholesterols and ionic strength of the solution, were studied. It was found that the fluorescence intensity of HB was sensitive to and also regulated by the microenvironments. When concentration of cholesterols and ionic strength keep invariable in PBS solution, there exists the maximum for the fluorescence of HB-liposome at pH 7.4 while the minimum for that of HB at pH 7.0. In addition, when pH value keeps constant (7.2), there exists the maximum at the ionic strength of 0.12 mol/kg while that at the concentration of 6×10⁻⁴ mol/L for cholesterols. On the other hand, in PBS solution, the lower the ionic strength is, the higher the fluorescence intensity is. The environment-sensitive fluorescence may be potentially applicable to probe some specific environmental features in cells or tissues.     

Study of fluorescence quenching and dialysis process of CdTe quantum dots, using ensemble techniques and fluorescence correlation spectroscopy

Luminescence properties of quantum dots (QDs) are closely related to their surface structure and chemical properties. In this work some ensemble techniques and fluorescence correlation spectroscopy (FCS) were used to study the fluorescence quenching and dialysis process of CdTe QDs. It is found that when some heavy metal ions, such as silver ions (Ag+), quench QDs, the free Ag+ ions bind with bare Te atoms and form the AgTe structure on the surface. The FCS experimental results show that the quenching process is not the gradual reduction of fluorescence intensity of single QDs, but the decrease in the number of bright QDs with the addition of Ag+ ions. In other words, the bright QDs turn into dark directly in the quenching process. It is observed that some dark QDs converse into the bright QDs in the dialysis experiments and the dialysis process can improve the brightness per QDs. Furthermore, the results of FCS and fluorescence spectroscopy illustrate that the increase of the fluorescence quantum yield (QY) is mainly attributed to the removal of excess unreacted Cd-MPA complex and the possible chemical change of the QDs surface in the dialysis process. These new results can help us to further understand the complex surface structure of water-soluble QDs, improve their surface chemical features, and expand their applications in some fields.