一种表征羟基自由基的新型荧光探针

表征羟基自由基 (· OH)的方法主要有电子自旋共振法[1] 和芳环羟基化法[2 ,3] 两大类 .电子自旋共振法灵敏度不高 ,且仪器设备昂贵 ,不适于常规分析 .芳环羟基化法操作较简单 ,灵敏度高 ,但芳环羟基化的产物往往不止一种 ,使得定量测定变得复杂 .其它方法如高效液相色谱法[4 ] ,化学发光法[5] 等也有报道 .顺磁性氮氧化合物能有效地清除自由基 [6 ,7] ,同时也是一种芳烃单重激发态的有效猝灭剂 [8,9] .当顺磁性氮氧化合物与荧光分子共价结合 ,所形成的荧光分子 -氮氧自由基复合物 (即自旋标记荧光分子 )仍保留对自由基反应的活性 ,但由于…     

Synthesis and spectral properties of polymethine-cyanine dye-nitroxide radical hybrid compounds for use as fluorescence probes to monitor reducing species and radicals

Various hybrid compounds comprised of two types of nitroxide radicals and either a pentamethine (Cy5) or trimethine cyanine (Cy3) were synthesized. The nitroxide radicals were linked either via an ester-bond to one or two N-alkyl carboxyl-terminated groups of Cy5, or via two amido-bonds (aminocarbonyl or carbonylamino group) to the 5-position of the indolenine moieties of Cy5 and Cy3. Changes in fluorescence and ESR intensities of the hybrid compounds were measured before and after addition of Na ascorbate in PBS (pH 7.0) to reduce the radicals. Among the hybrid compounds synthesized, those that linked the nitroxide radicals via an aminocarbonyl residue at the 5-position of the indolenine moieties on Cy5 and Cy3 exhibited a 1.8- and 5.1-fold increase in fluorescence intensity with the reduction of the nitroxide segment by the addition of Na ascorbate, respectively. In contrast, fluorescence intensity was not enhanced in the other hybrid compounds. Thus, the hybrid compounds which exhibited an increase in fluorescent intensity with radical reduction can be used in the quantitative measurement of reducing species such as Fe(2+) and ascorbic acid, and hydroxyl radicals. Because these hybrid compounds have the advantage of fluorescing at longer wavelengths-661 (Cy5) or 568 (Cy3)nm, respectively, they can be used to measure radical-reducing species or radicals either in solution or in vivo.     

Synthesis and properties of umbelliferone-nitroxide radical hybrid compounds as fluorescence and spin-label probes

Two hybrid compounds 6 and 7, linked via an ester-bond between the 7-hydroxyl residue of an umbelliferone 1 and a carboxylic acid residue of two nitroxide radicals 3 and 4, and one hybrid compound 8, linked via an ester-bond between a 3-carboxylic acid residue of umbelliferone 2 and a hydroxyl residue of nitroxide radical 5, were synthesized in good yields, and their fluorescence and ESR spectra before and after the addition of l-ascorbic acid sodium salt in PBS (pH 7.0) were measured. The ESR intensities of 6 and 7 were proportionally reduced after the addition of ascorbic acid sodium salt, and their fluorescence intensities were increased maximally by eight- and nine-fold, respectively. However, the fluorescence intensity of 8 was essentially unchanged.     

羟基自由基的流动注射荧光法测定

本文研究Fenton反应产生的·OH与Ce3+作用后Ce3+被氧化生成无荧光的Ce4+,通过测定Ce3+的荧光强度的下降可间接测定所产生的羟自由基,并结合流动注射技术,确定了体系最佳实验条件。同时测定抗氧化剂清除羟自由基的实验证明,该体系可作为在线筛选抗氧化剂以及在线测定羟自由基的方法。     

Determination of the antioxidant capacity of different food natural products with a new developed flow injection spectrofluorimetry detecting hydroxyl radicals

This paper presents an automatic spectrofluorimetric method (flow injection analysis spectrofluorimetry) for detecting hydroxyl radicals. Based on H₂O₂ catalyzed by Co²⁺ yielding HO, the method utilized sodium terephthalate to trap hydroxyl radicals and obtained sodium 2-hydroxyterephthalate by aromatic hydroxylation, which resulted in an increase in the fluorescence intensity. The relative fluorescence intensity was proportional to the concentration of hydroxyl radicals. Hydroxyl radicals could be determined indirectly, based on the increase of fluorescence. It was a simple, rapid, precise, sensitive and automatic technique for the determination of HO. The relative standard deviation of 11 determinations was 0.57%. The method can be used to sieve antioxidant medicines and will have theoretical and practical guidance on the mechanism of hydroxyl radicals-damaging biology.     

Quenching of cascade reaction between triplet and photochrome probes with nitroxide radicals

We proposed a new method for the study of molecular dynamics and fluidity of the living and model biomembranes and surface systems. The method is based on the measurements of the sensitized photoisomerization kinetics of a photochrome probe. The cascade triplet cis-trans photoisomerization of the excited stilbene derivative sensitized with the excited triplet Erythrosin B has been studied in a model liposome membrane. The photoisomerization reaction is depressed with nitroxide radicals quenching the excited triplet state of the sensitizer. The enhanced fluorescence polarization of the stilbene probe incorporated into liposome membranes indicates that the stilbene molecules are squeezed in a relatively viscous media of the phospholipids. Calibration of the "triple" cascade system is based on a previously proposed method that allows the measurement of the product of the quenching rate constant and the sensitizer's triplet lifetime, as well as the quantitative detection of the nitroxide radicals in the vicinity of the membrane surface. The experiment was conducted using the constant-illumination fluorescence technique. Sensitivity of the method using a standard commercial spectrofluorimeter is about 10(-12) mol of fluorescence molecules per sample and can be improved using an advanced fluorescence technique. The minimal local concentration of nitroxide radicals or any other quenchers being detected is about 10(-5) M. This method enables the investigation of any chemical and biological surface processes of microscopic scale when the minimal volume is about 10(-3) microL or less.     

Two-photon fluorescence microscopy imaging of cellular oxidative stress using profluorescent nitroxides

A range of varying chromophore nitroxide free radicals and their nonradical methoxyamine analogues were synthesized and their linear photophysical properties examined. The presence of the proximate free radical masks the chromophore's usual fluorescence emission, and these species are described as profluorescent. Two nitroxides incorporating anthracene and fluorescein chromophores (compounds 7 and 19, respectively) exhibited two-photon absorption (2PA) cross sections of approximately 400 G.M. when excited at wavelengths greater than 800 nm. Both of these profluorescent nitroxides demonstrated low cytotoxicity toward Chinese hamster ovary (CHO) cells. Imaging colocalization experiments with the commercially available CellROX Deep Red oxidative stress monitor demonstrated good cellular uptake of the nitroxide probes. Sensitivity of the nitroxide probes to H(2)O(2)-induced damage was also demonstrated by both one- and two-photon fluorescence microscopy. These profluorescent nitroxide probes are potentially powerful tools for imaging oxidative stress in biological systems, and they essentially "light up" in the presence of certain species generated from oxidative stress. The high ratio of the fluorescence quantum yield between the profluorescent nitroxide species and their nonradical adducts provides the sensitivity required for measuring a range of cellular redox environments. Furthermore, their reasonable 2PA cross sections provide for the option of using two-photon fluorescence microscopy, which circumvents commonly encountered disadvantages associated with one-photon imaging such as photobleaching and poor tissue penetration.     

A new approach for the detection of carbon-centered radicals in enzymatic processes using prefluorescent probes

In this communication we propose a novel application for prefluorescent probes in the detection of free carbon-centered radicals in enzymatic processes. Prefluorescent probes combine a fluorescent moiety tethered to a paramagnetic nitroxide that acts as a fluorescence quencher. Trapping of a radical by the nitroxide group restores the fluorescence properties. The increase in fluorescence intensity with time reflects the formation and quenching of carbon-centered radicals and can be used for the quantitative evaluation of yields and kinetics. As a test system we used horseradish peroxidase, an oxidoreductase that is widely accepted to operate by a radical-mediated mechanism. We used the prefluorescent probe (quinoline-TEMPO), where a quinoline moiety has been tethered to 2,2,6,6-tetramethylpiperidin-1-oxyl.     

Evaluation method of steric shielding effect around nitroxide radical reaction center based on molecular volume within a virtual ball

Steric shielding affects the stability of various molecules such as nitroxide radicals, which have many applications in a variety of fields. Thus, the mechanisms that maintain molecular stability are of particular interest. A new method for nitroxide radicals to quantify the steric shielding effect around the reaction center in a molecule was developed. The steric hindrance in this method is defined as the volume of the molecules contained within a virtual ball centered on the radical atom. With the proposed method, it is possible to evaluate the influences of the β-substituent, the basic molecular skeleton, and other parameters on steric hindrance, which cannot be calculated with E_s^c, a known parameter that indicates bulkiness. This method can acquire more accurate data that more closely resembles the behavior of the actual molecule. Because this method is very simple in that it requires only the optimal stable structure of the molecule, it can be used to estimate the steric shielding of various nitroxide radicals as well as other molecules.

     

水杨基荧光酮荧光法测定钴(Ⅱ)-过氧化氢体系产生 的羟自由基

本实验发现Co     

Determination of the rate constants of recombination of macroradicals and stable radicals via the competitive-inhibition method

The rate constants of recombination, k _X, of propagating radicals with nitroxides in pseudoliving radical polymerization are determined via the competitive-inhibition method with the use of ESR spectroscopy. This method is applicable to determination of k _X in the reactions of propagating radicals of styrene, acrylic acid, and methyl methacrylate with two stable radicals, the nitroxide diethylphosphono-2,2-dimethylpropyl nitroxide and the phenoxide galvinoxyl. The values of k _X determined at 50°C increase in the following sequence: diethylphosphono-2,2-dimethylpropyl nitroxide-TEMPO-galvinoxyl. The selectivity of the low-activity propagating radicals of styrene in reactions with stable radicals is shown.     

一个新的测定Fenton反应产生的·OH及清除的荧光方法

建立了一种测定羟基自由基的荧光新方法。Fenton反应产生的羟基自由基氧化二甲亚砜（DMSO）生成的甲醛与乙酰丙酮、氨发生Hantzsch反应，产物3，5－二乙酰－1，4－二氢吡啶产生特征荧光，其最大激发波长和最大发射波长分别为419.4nm和505.5nm。通过测定荧光强度的变化可以间接定量羟基自由基的产生量。该方法简便可靠，对于抗氧化剂的筛选以及羟基自由基的机理研究具有一定的应用价值。     

过氧亚硝酸诱导生成硫中心自由基的荧光表征

将4-羟基-2,2,6,6-四甲基哌啶氮氧自由基用于标记9-羧基-吖啶,得到自旋标记荧光探针4-(9-吖啶酯)-2,2,6,6-四甲基哌啶氮氧自由基. 以谷胱甘肽作为蛋白质肽模型,研究了活性氧过氧亚硝酸诱导其损伤产生的硫中心自由基的荧光表征. 自旋标记荧光探针为弱荧光物质,当与硫中心自由基作用后,导致其荧光增强,从而可对硫中心自由基进行表征.     

Flow injection fluorometric determination of ascorbic acid using perylenebisimide-linked nitroxide

A simple and sensitive flow injection fluorometric method for the determination of ascorbic acid is described. Perylenebisimide-linked nitroxide (PBILN) is used as a fluorescent reagent, which permits the selective determination of ascorbic acid. The fluorescence of the perylenebisimide moiety in PBILN is quenched by the nitroxide moiety, which is linked to the perylenebisimide. When a stream of a solution of ascorbic acid is merged with a stream of PBILN, the ascorbic acid reacts with the nitroxide moiety of PBILN to form hydroxylamine, and the fluorescence properties of the perylenebisimide moiety are recovered. As a result, a peak-shaped fluorescence signal is produced, which can be observed by a fluorescence detector located downstream. Under optimized conditions, a good linear relationship between the concentration of ascorbic acid and peak height in the concentration range from 0.5 to 10 μmol L⁻¹ was found and the detection limit (S/N = 3) was 0.28 μmol L⁻¹. The relative standard deviation for the determination of 4.0 μmol L⁻¹ ascorbic acid samples was 1.0% (n = 5). The proposed method was applied to the determination of ascorbic acid in several soft drink beverages and the analytical results were in good agreement with those obtained using a conventional method.     

A long-lived luminescence and EPR bimodal lanthanide-based probe for free radicals

We developed a novel spin-labeled terbium complex Tb(3+)/cs124-DTPA-TEMPO (1) by covalently labeling a nitroxide radical on the terbium complex for monitoring free radicals of various areas. This lanthanide complex probe shows a high EPR signal which resulted from the nitroxide radical moiety, and is weakly luminescent which resulted from the intramolecular quenching effect of the nitroxide radical on sensitised terbium luminescence. The intensity of both the EPR and luminescence can be modulated by eliminating the paramagnetism of the nitroxide radical through recognition of a carbon-centered radical analyte and thus gives a quantification of the analyte. We have preliminarily applied this probe in the luminescent detection of model carbon-centered radicals and hydroxyl radicals (·OH). This probe is water-soluble and contains lanthanide-luminescence properties, favorable for the time-resolved luminescence technique. The investigation of the intramolecular quenching process has showed that the labeled nitroxide radical quenches multiple excited states of the terbium complex, resulting in highly efficient quenching of terbium luminescence. This probe is the first example of intramolecular modulation of lanthanide luminescence by a nitroxide radical.     

苯基荧光酮光度法测定·OH

建立了一种新的测定Fenton反应所产生的羟自由基的方法 ,苯基荧光酮 (Phenylfluorone ,简称本芴酮 )与Fenton试剂作用后 ,使其荧光大大降低 ,其最大激发波长和发射波长分别为 50 0nm和 42 0nm ,基于苯基荧光酮在反应前后的荧光变化 ,即可间接地测定羟自由基的产生量。同时 ,通过清除率实验反证了该方法的可靠性 ,利用顺磁共振法测定苯基荧光酮加入前后的波谱变化来进一步证实该方法的正确性。化学测定过程均在国产仪器下完成 ,具有较高的灵敏度。可推广为一种作为寻找羟自由基清除剂的方法 ,也可作为医学上部分药品性能检验的一种方法     

Nitroxides scavenge myeloperoxidase-catalyzed thiyl radicals in model systems and in cells

Nitroxide radicals possess important antioxidant activity in live tissues because of their ability to scavenge reactive radicals. Despite the fact that, in cells, damaging free radicals are primarily quenched by glutathione (GSH) with subsequent formation of harmful glutathionyl radical (GS(*)), interactions of nitroxide radicals with GS(*) and thiols have not been studied in detail. In addition, intracellular metabolic pathways leading to the formation of secondary amines from nitroxides are unknown. Here we report that GS(*) radicals react efficiently and irreversibly with nitroxides to produce secondary amines. We developed a sensitive method for the detection of GS(*) based on their specific interaction with Ac-Tempo, a nonfluorescent conjugate of fluorogenic acridine with paramagnetic nitroxide Tempo, and used it to characterize interactions between nitroxide and thiyl radicals generated through phenoxyl radical recycling by peroxidase. During reaction of Ac-Tempo with GS(*), Tempo EPR signals decayed and acridine fluorescence concurrently increased. DMPO and PBN, spin traps for GS(*), inhibited this interaction. Using combined HPLC and mass spectrometry, we determined that 90% of the Ac-Tempo was converted into fluorescent acridine (Ac)-piperidine; GSH was primarily oxidized into sulfonic acid. In myeloperoxidase-rich HL-60 cells, Ac-piperidine fluorescence was observed upon stimulation of GS(*) generation by H(2)O(2) and phenol. Development of fluorescence was prevented by preincubation of cells with the thiol-blocking reagent N-ethylmaleimide as well as with peroxidase inhibitiors. Furthermore, Ac-Tempo preserved intracellular GSH and protected cells from phenol/GS(*) toxicity, suggesting a new mechanism for the free-radical scavenging activity of nitroxides in live cells.     

A new method to study antioxidant capability: hydrogen transfer from phenols to a prefluorescent nitroxide

[reaction: see text]. Rate constants for hydrogen abstraction from phenols by a prefluorescent-TEMPO probe are reported. The nitroxide is employed as a potential model of peroxyl radicals. The probe works by nitroxide suppression of the fluorescence of the chromophore. The fluorescence is restored when the nitroxide abstracts a hydrogen atom to produce the diamagnetic hydroxylamine. The phenols studied in this project exhibited rate constants between 0.003 and 0.2 M(-1) s(-1). A deuterium isotope effect of 10 for TROLOX confirms that the mechanism is dominated by hydrogen transfer.     

Energy transfer in polymers and nitroxide decay during photolysis

When polymeric materials doped with nitroxides of the 2,2,6,6-tetramethylpiperidine type are exposed to light, the nitroxide concentration decreases. The two mechanisms for the decrease of the nitroxide are the reaction of nitroxide with free radicals produced during photolysis of the polymer to form amino ethers and the abstraction of hydrogen atoms by excited-state nitroxides to form hydroxyl amines. Excited-state nitroxides can be formed in two ways: by direct absorption and by energy transfer. In this paper, the effect of energy transfer on the rate of decay of the nitroxide signal is studied, and measurements of nitroxide decay are used to probe energy transfer in crosslinked polymeric coatings. A simple kinetic scheme is used to interpret nitroxide decay during photolysis of both solutions and polymers containing benzophenone. These results are used to show that the slope of the line relating nitroxide decay rate to nitroxide concentration is essentially determined by energy transfer from a coating-based chromophore to nitroxide. The nitroxide decay assay is also used to study the effectiveness of a benzotriazole ultraviolet light absorber as a quencher.     

The spectrofluorqmetric determination of anthracene, fluorene and phenanthrene in mixtures

A procedure is presented for the spectrofluorometric determination of mixtures of anthracene, fluorene and phenanthrene. The determination depends on differences in fluorescence emission spectra and on selective excitation of anthracene fluorescence. Some of the fluorescence and absorption spectra involved overlap, but these difficulties can be overcome by empirical corrections. The average relative error in this method is less than 5 % over the concentration range 0 to 5 ppm.