Gold nanoparticles-based catalysis for detection of S-nitrosothiols in blood serum

Accumulating evidence suggests that S-nitrosothiols (RSNOs) play key roles in human health and disease. To clarify their physiological functions and roles in diseases, it is necessary to promote some new techniques for quantifying RSNOs in blood and other biological fluids. Here, a new method using gold nanoparticle catalysts has been introduced for quantitative evaluation of RSNOs in blood serum. The assay involves degrading RSNOs using gold nanoparticles and detecting nitric oxide (NO) released with NO-selective electrodes. The approach displays very high sensitivity for RSNOs with a low detection limit in the picomolar concentration range (5.08 × 10⁻¹¹ mol L⁻¹, S/N = 3) and is free from interference of some endogenous substances such as NO₂⁻ and NO₃⁻ co-existing in blood serum. A linear function of concentration in the range of (5.0-1000.0) × 10⁻⁹ mol L⁻¹ has been observed with a correlation coefficient of 0.9976. The level of RSNOs in blood serum was successfully determined using the described method above. In addition, a dose-dependent effect of gold nanoparticles on the sensitivity for RSNOs detection is revealed, and thereby the approach is potentially useful to evaluate RSNOs levels in various biological fluids via varying gold nanoparticles concentration.     

Quantitation of Cu+‐catalyzed Decomposition of S‐Nitrosoglutathione Using Saville and Electrochemical Detection: a Pronounced Effect of Glutathione and Copper Concentrations

S‐nitrosothiols (RSNOs) are composed of nitric oxide (NO) bound to the sulfhydryl group of amino acids of peptides or proteins. There is a great interest for their quantitation in biological fluids as they have a crucial impact on physiological and pathophysiological events. Most analytical methodologies for quantitation of RSNOs are based on their decomposition followed by the detection of the released NO. In order to obtain the optimal sensitivity for each detection method, the total decomposition of RSNOs is highly desired. The decomposition of RSNOs can be obtained by using catalytically active metal ions, such as Cu⁺, obtained from CuSO₄ in presence of a reducing agent such as glutathione (GSH) that is naturally present in biological environment. In this work, we have re‐investigated the decomposition of S‐nitrosoglutathione (GSNO) which is the most abundant in vivo low molecular weight RSNO, with a special emphasis on the effect of CuSO₄, GSH, and GSNO concentrations and of their ratio. To this aim, GSNO decomposition optimization was performed by both indirect (Griess assay) and direct (real time electrochemical detection of NO at NO‐microsensor) quantitation methods. Our results show that the ratio between CuSO₄, GSH and GSNO should be adjusted to tune the highest decomposition rate of GSNO and the most efficient electrochemical detection of released NO; also it shows the deleterious effect of very high GSH concentration on the detection of GSNO.     

A New Ultramicrosensor for Nitric Oxide Based on Electropolymerized Film of Nickel Salen

Abstract

A new amperometric ultramicrosensor for the determination of nitric oxide (NO) is described. The ultramicrosensor, which is based on an electropolymerized film of ethylenebis(salicylideneiminate) nickel [Ni(salen)] and Nafion, shows a low detection limit, high selectivity and sensitivity to NO determination. The oxidation current (measured by a differential pulse amperometric method) is linear with NO concentration ranging from 1.0x10^?8 to 4.0x10^?6 mol/L with a calculated detection limit, at a signal to noise ratio of three, equal to 5.0x10^?9 mol/L. Some endogenous electroactive substances in biological tissues, such as dopamine, 5-HT and nitrite do not interfere with NO determination at the concentrations higher than those in biological systems. The ultramicrosensor could be employed for in vivo measurements of NO. The mechanism of the response of the ultramicrosensor to NO is also studied.     

Enhanced flow injection analysis for measurements of S-nitrosothiols species in biological samples using highly selective amperometric nitric oxide sensor

A highly selective nitric oxide(NO) sensor is fabricated and applied to devise an enhanced flow injection analysis(FIA) system for S-nitrosothiols(RSNOs) measurement in biological samples.The NO sensor is prepared using a polytetrafluoroethylene(PTFE) gas-permeable membrane loaded with Teflon AF? solution,a copolymer of tetrafluoroethylene and 2,2-bis(trifluoroethylene)-4,5-difluoro -l,3-dioxole,to improve selectivity.This method is much simpler and possesses good performance over a wide range of RSNOs concentrations.Standard deviation for three parallel measurements of blood plasma is 4.0%.The use of the gas sensing configuration as the detector enhances selectivity of the FIA measurement vs.using less selective electrochemical detectors that do not use PTFE/Teflon type outer membranes.     

Flow injection measurements of <Emphasis Type="Italic">S</Emphasis>-nitrosothiols species in biological samples using amperometric nitric oxide sensor and soluble organoselenium catalyst reagent

A novel flow injection analysis (FIA) system suitable for measurement of S-nitrosothiols (RSNOs) in blood plasma is described. In the proposed (FIA) system, samples and standards containing RSNO species are injected into a buffer carrier stream that is mixed with the reagent stream containing 3,3′-dipropionicdiselenide (SeDPA) and glutathione (GSH). SeDPA has been shown previously to catalytically decompose RSNOs in the presence of a reducing agent, such as GSH, to produce nitric oxide (NO). The liberated NO is then detected downstream by an amperometric NO sensor. This sensor is prepared using an electropolymerized m-phenylenediamine (m-PD)/resorcinol and Nafion composite films at the surface of a platinum electrode. Using optimized flow rates and reagent concentrations, detection of various RSNOs at levels in the range of 0.25–20 μM is possible. For plasma samples, detection of background sensor interference levels within the samples must first be carried out using an identical FIA arrangement, but without the added SeDPA and GSH reagents. Subtraction of this background sensor current response allows good analytical recovery of RSNOs spiked into animal plasma samples, with recoveries in the range of 90.4–101.0%.     

A Novel Nitric Oxide Cellular Biosensor Based on Red Blood Cells Immobilized on Gold Nanoparticles

Abstract

We have developed a novel nitric oxide (NO) cellular biosensor based upon the immobilization of red blood cells (RBCs) onto nanometer‐size colloidal gold that is attached to an electrochemically pretreated glassy carbon electrode via the bridging of an ethylenediamine monolayer. The biosensor has been characterized by atomic force microscopy (AFM), scanning electron microscopy (SEM), and electrochemistry. The immobilized RBCs display an excellent electrocatalytic response to nitric oxide. The electrocatalytic currents are proportional to the NO concentration in the range from 1.0×10^–8 to 1.0×10^–6 M and the detection limit is as low as 5.0×10^–9 M (S/N=3). Furthermore, the biosensor is very stable and relatively free of potential interference.     

A novel electrochemical microsensor for the determination of NO and its application to the study of the NO donor S-nitrosoglutathione

A novel electrochemical microsensor for the determination of NO based on an electropolymerized film of tetraaminophthalocyaninecopper [Cu(TAPc)] was prepared. Its response to NO and its application to the study of an NO donor (S-nitrosoglutathione; GSNO) are also described. The microsensor exhibited an electrocatalytic effect on NO oxidation and showed a low detection limit, high sensitivity and selectivity for NO determination. The oxidation current (measured by differential pulse amperometry) was linear for NO concentrations ranging from 6.2 x 10(-9) to 3.0 x 10(-5) mol L-1 with a calculated detection limit of 4.0 x 10(-9) mol L-1 (S/N = 3) and a linear coefficient of 0.9984. Some endogenous electroactive substances in biological tissues, such as dopamine, 5-hydroxytryptamine and nitrite, at concentrations higher than those in biological systems did not interfere with NO determination. The sensor shows promise for the possible in vivo determination of NO. Using the microsensor, the NO release from the NO donor (GSNO) was successfully monitored. This work sets a foundation for the study of the pharmacology and the biological effects in vivo of S-nitrosothiols.     

A Nitric Oxide Biosensor Based on Myoglobin Adsorbed on Multi‐Walled Carbon Nanotubes

Myoglobin (Myb) of horse heart is incorporated on multi‐walled carbon nanotubes (MWNTs) and immobilized at a glassy carbon (GC) electrode surface. Its electrochemical behavior and enzyme activity are characterized by employing electrochemical methods. The results indicate that MWNTs can obviously promote the direct electron transfer between Myb and electrode, and that the Myb on MWNTs behaves as an enzyme‐like activity towards the electrochemical reduction of nitric oxide (NO). Accordingly, an unmediated NO biosensor is constructed. Experimental results reveal that the peak current related to NO is linearly proportional to its concentration in the range of 2.0×10^?7–4.0×10^?5 mol/L. The detection limit is estimated to be 8.0×10^?8 mol/L. Considering a relative standard deviation of 2.1% in seven independent determinations of 1.0×10^?5 mol/L NO, this biosensor shows a good reproducibility. The biosensor based on Myb/MWNTs modified electrode can be used for the rapid determination of trace NO in aqueous solution with a good stability, nice selectivity and easy construction.     

Oxidation Mechanisms of NAD(P)H Model Hantzsch 1,4-Dihydropyridines by RSNO

The important roles of nitric oxide (NO) in adjusting many physiological functions in life processes have attract ed considerable attention of many researchers over the past twenty years.[1] S-Nitrosothiols (henceforth called RSNOs) have been detected in vivo, and they are currently believed to be responsible for storing and transporting NO.[2] NAD(P)H is a typical redox coenzyme which plays an important role in NO synthesis and transfer from RSNOs in vivo. So it is interesting to investigate the reaction of RSNOs and NAD(P)H. In previous paper,[3] Professor Wu reported the reaction of GSNO with Hantzsch esters. In this paper our focus is on the kinetics of the reac tion of 4-substitued Hantzsch esters with Ph3CSNO (Eq. 1).     

Real-time measurement of nitric oxide using a bio-imaging and an electrochemical technique

Nitric oxide (NO) is an important mediator responsible for numerous physiological phenomena. Transient levels of NO in biological systems usually range from nanomolar to micromolar concentrations, with a rapid return to basal levels normally seen following these increases. Because NO can diffuse only over a local area in limited time due to such low levels of production and due to its short life-time prior to degradation, high spatial and temporal resolutions are required for direct and continuous NO measurement if the physiological role of NO is to be investigated in any system. For such purposes, analytical methods based on bio-imaging and electrochemical techniques for the measurement of NO are useful. In this paper, we describe the successful application of these methods to a number of biological systems. Specifically, complementary application of these methods demonstrate that it is possible to detect real-time NO production from nervous tissue with high spatial and temporal resolutions.     

Determination of S-nitrosoglutathione and other nitrosothiols by p-hydroxymercurybenzoate derivatization and reverse phase chromatography coupled with chemical vapor generation atomic fluorescence detection

S-Nitrosoglutathione (GSNO) reacts with the organic mercurial probe, p-hydroxymercury benzoate (PHMB, HO-Hg-(C₆H₄)-COO⁻Na⁺) giving the complex GS-Hg(C₆H₄)COOH (GS-PHMB). This reaction has been studied by UV measurements at 334 nm also in the presence of ascorbic acid and the product of reaction, the GS-PHMB complex, characterized by Electrospray Ionization Mass Spectrometry (ESI-MS) and by Reversed Phase Chromatography (RPLC) coupled on-line and sequentially with a UV-visible diode array detector (DAD) followed by a cold vapor generation atomic fluorescence spectrometer (CVGAFS). The simultaneous presence of PHMB and ascorbate produced a synergistic effect on GSNO decomposition rate that can be observed only above a given concentration threshold of ascorbate (ascorbate/GSNO molar ratio ≥ 180). The results indicated that the formation of GS-PHMB, both in the presence and the absence of ascorbic acid, does not involve the formation of free thiolic species but it takes place through a more complex mechanism. The PHMB derivatives of GSH and GSNO obtained by the present method were found to be identical by ESI-MS. GSSG did not interfere because it was not reduced and derivatized to GS-PHMB. Once complexed by the alkylating agent N-ethylmaleimide (NEM), GSH did not interfere with the derivatization reaction. This ensured a good selectivity of the developed PHMB derivatization system for RSNO determination. Thus, we have optimized the operating conditions for the selective reaction of PHMB with GSNO and other nitrosothiols (RSNOs) in order to determinate RSNOs in human plasma. LODc for RSNOs in plasma ultrafiltrate was 30 nM (injected concentration, 50 μL loop), the DLR ranged between 0.08 and 50 μM and the CV% was 6.5% at 300 nM concentration level. Reduced and oxidized thiols spiked to plasma did not interfere with the measurement of RSNOs. We found that the sampling procedure was critical for the recovery of endogenous and spiked RSNOs. The ultrafiltrate samples of plasma of 8 healthy humans contained 1460 ± 310 CysNO, 1000 ± 330 nM HCysNO and 320 ± 60 nM GSNO if blood was sampled in a mixture NEM/ethylendiaminotetracetic acid (EDTA)/serine-borate complex (SBC), where serine-borate complex is a potent inhibitor of γ-glutamyltransferase, an enzyme involved in the conversion of GSNO into CysGlyNO. In the absence of SBC during the sampling of blood GSNO concentration found in the ultrafiltrate was lower (at level of the determination limit in plasma ultrafiltrate, i.e. 75 nM) and the peak of CysGlyNO appeared, which corresponded to a concentration of 200 ± 60 nM (N = 4 blood samples).     

Detection of nitric oxide in single cells

Nitric oxide (NO) is endogenously generated by nitric oxide synthase (NOS) enzymes and is involved in a surprisingly wide range of biological functions. As efforts are made to elucidate the regulatory mechanisms of NOS expression and function, there is increasing interest in following NOS activity directly by monitoring NO production. Additionally, spatial and temporal measurements of NO are important for understanding its function and metabolism. In this work, developments in technology enabling NO detection in biological systems are reviewed. Measuring NO at single cell levels is important as NOS is heterogeneously distributed; however, such measurements are difficult as physiological NO levels are in the low nanomolar to low micromolar range. Here, three categories of analytical techniques enabling NO detection at single cell levels are highlighted: fluorescence microscopy, capillary electrophoresis with laser induced fluorescence detection, and electrochemistry. For each, the basic principles, performance, applications, figures of merits and limitations are presented in terms of single cell NO detection.     

Voltammetric Behavior of Sodium 7-Methoxyl-4＇-hydroxylisoflavone-3＇-sulfonate and Its Application

Voltammetric behavior of sodium 7‐methoxyl‐4′‐hydroxylisoflavone‐3′‐sulfonate (SMHS) in the aqueous solution from pH 1 to 5 was studied by linear sweep voltammetry, cyclic voltammetry and normal pulse voltammetry. Experimental results showed that in 0.2 mol*L^?1 sodium citrate‐hydrochloric acid buffer solution (pH=4.65), SMHS caused only one reduction wave at ?1.34 V (vs. saturated calomel electrode, SCE), which was an h‐reversible adsorptive wave of SMHS protonized involving one electron and one proton. The peak current of SMHS on linear sweep voltammogram was proportional to its concentration in the range of 8.0 × 10 ?8.0·10 mol*L^?1 (r = 0.995). and the detection limit was 5.0·10^?‐⁶mol*L^?1. The method was applied to determination of SMHS, in synthetic samples. In addition, its scavenging effect on superoxide anion radical was studied by the auto‐oxidation of pyrogallol in HCI‐tris buffer solution (pH = 8.2) in order to explain its peculiar biological effects. The experimental results proved that SMHS has antioxidant quality, and it is an efficient free radical scavenger of superoxide anion radical.     

一氧化氮在大环铜配合物修饰电极上的电催化氧化及测定

发现大环铜配合物 [Cu(Ⅱ )L]Cl2对一氧化氮（ NO）具有电催化氧化作用（ L=1, 8 - 二乙醇基 - 1, 3, 6, 8, 10, 13 - 六氮杂 - 14 - 冠 - 4） ; 研制成用于 NO伏安法测定的微铂盘 Nafion－ Cu(Ⅱ )L膜修饰电极。当 NO 的浓度在 1.4× 10－ 5 ～ 5.6× 10－ 7 mol/L范围内氧化峰电流与 NO的浓度呈线性关系,相关系数为 0.994,亚硝酸、抗坏血酸、多巴胺等物质不干扰 NO测定。     

4-Aryl-1,3,2-oxathiazolylium-5-olates as pH-controlled NO-donors: the next generation of S-nitrosothiols

S-Nitrosothiols (RSNOs) are important exogenous and endogenous sources of nitric oxide (NO) in biological systems. A series of 4-aryl-1,3,2-oxathiazolylium-5-olates derivatives with varying aryl para-substituents (-CF3, -H, -Cl, and -OCH3) were synthesized. These compounds were found to release NO under acidic condition (pH = 5). The decomposition pathway of the aryloxathiazolyliumolates proceeded via an acid-catalyzed ring-opening mechanism after which NO was released and an S-centered radical was generated. Electron paramagnetic resonance (EPR) spin trapping studies were performed to detect NO and the S-centered radical using the spin traps of iron(II) N-methyl-D-glucamine dithiocarbamate [(MGD)2-FeII] and 5,5-dimethyl-1-pyrroline N-oxide (DMPO). Also, EPR spin trapping and UV-vis spectrophotometry were used to analyze the effect of aryl para substitution on the NO-releasing property of aryloxathiazolyliumolates. The results showed that the presence of an electron-withdrawing substituent such as -CF3 enhanced the NO-releasing capability of the aryloxathiazolyliumolates, whereas an electron-donating substituent like methoxy (-OCH3) diminished it. Computational studies using density functional theory (DFT) at the PCM/B3LYP/6-31+G**//B3LYP/6-31G* level were used to rationalize the experimental observations. The aryloxathiazolyliumolates diminished susceptibility to reduction by ascorbate or gluthathione, and their capacity to cause vasodilation as compared to other S-nitrosothiols suggests potential application in biological systems.     

Molecular Diffusion Measurement in Lipid Bilayers over Wide Concentration Ranges: A Comparative Study

Molecular diffusion in biological membranes is a determining factor in cell signaling and cell function. In the past few decades, three main fluorescence spectroscopy techniques have emerged that are capable of measuring molecular diffusion in artificial and biological membranes at very different concentration ranges and spatial resolutions. The widely used methods of fluorescence recovery after photobleaching (FRAP) and single‐particle tracking (SPT) can determine absolute diffusion coefficients at high (>100 μm^?2) and very low surface concentrations (single‐molecule level), respectively. Fluorescence correlation spectroscopy (FCS), on the other hand, is well‐suited for the intermediate concentration range of about 0.1–100 μm^?2. However, FCS in general requires calibration with a standard dye of known diffusion coefficient, and yields only relative measurements with respect to the calibration. A variant of FCS, z‐scan FCS, is calibration‐free for membrane measurements, but requires several experiments at different well‐controlled focusing positions. A recently established FCS method, electron‐multiplying charge‐coupled‐device‐based total internal reflection FCS (TIR‐FCS), referred to here as imaging TIR‐FCS (ITIR–FCS), is also independent of calibration standards, but to our knowledge no direct comparison between these different methods has been made. Herein, we seek to establish a comparison between FRAP, SPT, FCS, and ITIR–FCS by measuring the lateral diffusion coefficients in two model systems, namely, supported lipid bilayers and giant unilamellar vesicles.     

Glutathione Peroxidase‐Based Amperometric Biosensor for the Detection of S‐Nitrosothiols

A new biosensor is described for the detection of S‐nitrosothiols (RSNOs) based on their decomposition by immobilized glutathione peroxidase (GPx), an enzyme containing selenocysteine residue that catalytically produces nitric oxide (NO) from RSNOs. The enzyme is entrapped at the distal tip of a planar amperometric NO sensor. The new biosensor shows good sensitivity, linearity, reversibility, and response times towards various RSNO species in PBS buffer, pH 7.4 . In most cases, the response time is less than 5 min, and the response is linear up to 6 μM of the tested RSNO species. The lowest detection limit is obtained for S‐nitrosocysteine (CysNO), at approx. 0.2 μM. The biosensor's sensitivity is not affected by the addition of EDTA as a chelating agent; an advantage over other potential catalytic enzymes that contain copper ion centers, such as CuZn‐superoxide dismutase and xanthine oxidase. However, lifetime of the new sensor is limited, with sensitivity decrease of 50% after two days of use. Nonetheless, the new amperometric GPx based RSNO sensor could prove useful for detecting relative RSNO levels in biological samples, including whole blood.     

Evidence of polyphenols nitrosation by computer aided ESR spectroscopy

Polyphenols play an important role as model systems in transition metal derivatives for the preparation of macromolecular systems. Among the metal ions ironnitrosyl coordination chemistry has received much attention in the past because of its important role in inorganic and biological processes. In the case of Fe(I)(NO)₂ complexes with polyphenols ligands in solution, difficulties in the interpretation of the ESR spectra arise from complicated patterns due to simultaneous presence of different nitrogen nuclei directly bound to the metal ion or due to the presence of equilibria between species under slow exchange conditions. In order to overcome these difficulties the investigations reported here were carried out using computer simulation of ESR spectra combined with selective isotopic substitution of ¹⁴NO with ¹⁵NO. Resorcinol displays an unexpected nine lines ESR pattern at g=2.018 which can be explained only by considering more than two nitrogen atoms interacting with the unpaired electron delocalized over the metal complex.     

可释放一氧化氮聚合物材料的制备及其在生物医疗器械中的应用

一氧化氮（NO）是一种很好的血小板黏附或活化的抑制剂，同时也是很有效的抗平滑肌细胞增生剂。可释放NO的聚合物材料显示出较好的抗血栓形成及抑制细胞增生的性能。本文综述了可释放NO聚合物材料的制备方法及其近年来在生物医疗器械中的应用。用来制备可释放NO聚合物材料的NO供体主要有两大类，一类是亲核NO供体N-diazeniumdiolates，另一类是S-亚硝基硫醇（RENOs）。制备可释放NO聚合物材料的方法主要有3种：（1）通过物理掺杂的方式将小分子的NO供体分散到聚合物材料中；（2）对聚合物材料的填料微粒进行化学改性，得到可释放NO的填料粒子，再将其填充到聚合物材料中；（3）通过共价键将可释放NO的基团连接到聚合物主链及侧链上。所得到的可释放NO聚合物材料在血管内传感器、体外血液循环电路和体内移植血管等生物医疗器械中有广泛的应用。