Detection of naphthalene sulfonates from highly saline brines with high-performance liquid chromatography in conjunction with fluorescence detection and solid-phase extraction

A procedure is developed for the simultaneous determination of 1-naphthalene sulfonate, 2-naphthalene sulfonate, 1,5-naphthalene disulfonate, 1,6-naphthalene disulfonate, 2,6-naphthalene disulfonate and 2,7-naphthalene disulfonate from highly saline geothermal brines using ion-pair high-performance liquid chromatography with fluorescence detection after solid-phase extraction. The substances are baseline separated within 33 min and recoveries in brines with salinities of up to 175?g/L NaCl are 100%?(±?10) by solid-phase extraction. For the overall method, the method quantification limits of the analytes are between 0.05 and 0.4?μg/L. The method is also shown to be feasible for matrices encountered in deep geothermal reservoirs.     

Evaluation of densitometric quantitation of ether phospholipids by high performance thin layer chromatography

Summary This paper reports on the use of uni-dimensional high performance thin layer chromatography on silica gel for the separation and detection of ether phospholipids involving in situ reflectance densitometry. Dipping reagents for charring (cupric sulfate-phosphoric acid and manganese chloride-sulfuric acid) or fluorescence enhancement (1-anilino-8-naphthalene sulfonate) were evaluated. Two lipophilic fluorescence reagents (2,5-bis-5′-tert-butylbenzoxazolyl-(2′))thiophene and 4-(N,N-dihexadecyl)amino-7-nitrobenz-2-oxa-1,3-diazole) which move in the mobile phase were tested. The latter reagent gave the more sensitive and stable measurements: nanogram amounts of ether phospholipids could be detected in a reproducible way. Since alkyl lysophospholipids are highly polar molecules, high performance thin layer chromatography is a challenge. Characteristics of sorbents and influence of mobile phases on detection and separation are discussed for the NBD-dihexadecylamine fluorescence detection method.     

2-(p -toluidino)-6-naphthalene sulfonate as a fluorescent probe for flocculation studies of cationic potato amylopectin and nanosized silica particles. 2. Flocculation by binding of nanosized silica particles

2-(p-toluidino)-6-naphthalene sulfonate (TNS) is a probe that fluoresces strongly when bound to certain proteins and polymers, but weakly in aqueous solutions. The reversible association of TNS is used to monitor the binding of anionic nanosized silica particles (NSP) to cationic potato amylopectin starch (CApS) through the decreasing fluorescence emission as TNS is competitively released by the particle binding. Steady-state fluorescence measurements at different mixing ratios of CApS and NSP provide data on the equilibrium binding. The isotherm derived is used to establish the fact that the most efficient flocculation between CApS and NSP occurs when the polymer coils are nearly saturated by NSP, but still have positively charged parts left. This supports a patch-flocculation mechanism. Stopped-flow experiments show that NSP binding to CApS occurs within a few milli seconds. This observation allows turbidity changes which occur on longer timescales to be ascribed to particle-decorated polymers undergoing changes in the conformation or aggregation. Received: 14 August 1998 Accepted in revised form: 4 December 1998     

Trace determination and characterization of some proteins in blood serum by high-performance liquid chromatography with a time-resolved laser fluorimetric detector

Protein in human serum is measured by high-performance liquid chromatography with a time- resolved laser fluorimetric detector. The detection limit is 2.3 pmol for bovine serum albumin; the value is governed by fluctuation of the background fluorescence from free 1-anilino-8-naphthalene sulfonate (ANS) used as the fluorescence probe. Micropolarity of the binding site in protein is estimated by measuring the fluorescence lifetime of ANS bound to protein; the micropolarity for albumin is lower than those for α- and γ-globulins.     

Polyelectrolyte titration using fluorescent indicator. I. Direct titration of anionic and cationic polyelectrolytes with 10−4N standard solutions

The polyelectrolyte titration, which was originally called colloid titration, is based on the stoichiometric reaction between positively charged colloidal particles and negatively charged ones. In the conventional method, the metachromatic color change of the indicator, toluidine blue, from blue to red-purple has been applied for the determination of the end point in the titration. 2.5 × 10^?3N potassium polyvinylsulfonate (KPVS) is usually used as the standard titrant. In this work, fluorescent indicators such as 6-(p-toluidino)-2-naphthalene sulfonate (TNS), acridine orange, etc., have been introduced. The fluorescence intensity was measured using the spectrophotometer equipped with magnetic stirrer and connected with a vinyl tube attached to the hand piston burette. For example, TNS is practically nonfluorescent, but it exhibits strong fluorescence when it is bound to a cationic polyelectrolyte (CP). The fluorescence of the TNS–CP complex is diminished by titration with KPVS standard solution since TNS is liberated from the complex by substitution with KPVS. After the equivalent point, the fluorescence intensity becomes constant and the end point can thus be detected by that point. It has been elucidated that the very dilute standard solution like 1 × 10^?4N can be used because the sensitivity of fluorescence detection is extremely high. © 1993 John Wiley & Sons, Inc.     

2-(p-toluidino)-6-naphthalene sulfonate as a fluorescent probe for flocculation studies of cationic potato amylopectin and nanosized silica particles 1. 2-p-(toluidino)-6-naphthalene sulfonate binding to cationic amylopectin

2-(p-toluidino)-6-naphthalene sulfonate (TNS) is a probe that fluoresces strongly when bound to certain proteins and polymers, but weakly in aqueous solution. Absorption and fluorescence spectroscopy were used to study the interaction of TNS with native amylopectin potato starch (NApS) and cationized amylopectin potato starch (CApS) in aqueous solution. The anionic TNS binds to CApS at a single type of binding site, with an affinity which has both electrostatic and nonelectrostatic contributions (including hydrogen bonding), whereas binding to NApS occurs at the same type of site but only by nonelectrostatic means. The affinity to CApS decreases strongly with increasing salt concentration, due to screening of the electrostatic attraction, whereas with NApS increasing salt concentration slightly enhances the binding affinity, most likely due to screening of a weak repulsive interaction between TNS and phosphate residues on NApS. The association constant for binding of TNS to CApS in 5 mM NaCl is 110 ± 20 M⁻¹. This comparatively weak binding makes TNS a useful probe in kinetic investigations of the flocculation of anionic silica particles by CApS. Received: 14 August 1998 Accepted in revised form: 4 December 1998     

Quantitative evaluation of thin-layer chromatograms by means of the solvatochromic fluorescence of 8-(phenylamino)-1-naphthalenesulfonate

Summary Polarity dependent fluorescence of 8-(phenylamino)-1-naphthalene sulfonate (8,1 ANS) was used to develop a quantitative evaluation method for thin-layer chromatograms (TLCs). After the compounds have been separated the dye is applied to the chromatogram where it is extracted by the substances and shows — upon excitation — a significant fluorescence. This is a way to quantify photophysically inactive molecules without preceding derivatization. Fluorescence intensity correlates well with the amount of the compounds as is shown in the cases of three wax components.

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Quantitative Auswertung von Dünnschicht-Chromatogrammen mit Hilfe der solvatochromen Fluorescenz von 8-(Phenylamino)-1-naphthalin-Sulfonat

     

Indirect Fluorimetric Detection of Cyclodextrins via Postcolumn Mixing with 2-p-Toluidinyl-6-naphthalenesulfonate in Liquid Chromatography

Cyclodextrins (CD's) were visualized by postcolumn mixing with 2-p-toluidinylnaphthalene sulfonate (TNS) in liquid chromatography. The indirect detection is based on fluorescence enhancement due to the formation of an inclusion complex between TNS and CD's. β-CD gave larger signal intensity than α- and γ-CD. Different selectivities were observed for alkyl-bonded silica stationary phases with different chain length.     

Identification of Folding Intermediates of Streblin,The Most Stable Serine Protease: Biophysical Analysis

Streblin, a serine proteinase from plant Streblus asper, has been used to investigate the conformational changes induced by pH, temperature, and chaotropes. The near/far UV circular dichroism activities under fluorescence emission spectroscopy and 8-aniline-1-naphthalene sulfonate (ANS) binding have been carried out to understand the unfolding of the protein in the presence of denaturants. Spectroscopic studies reveal that streblin belongs to the α+β class of proteins and exhibits stability towards chemical denaturants, guanidine hydrochloride (GuHCl). The pH-induced transition of this protein is noncooperative for transition phases between pH 0.5 and 2.5 (midpoint, 1.5) and pH 2.5 and 10.0 (midpoint, 6.5). At pH 1.0 or lower, the protein unfolds to form acid-unfolded state, and for pH 7.5 and above, protein turns into an alkaline denatured state characterized by the absence of ANS binding. At pH 2.0 (1 M GuHCl), streblin exists in a partially unfolded state with characteristics of a molten globule state. The protein is found to exhibit strong and predominant ANS binding. In total, six different intermediate states has been identified to show protein folding pathways.     

Studies on the Toluidine Blue Dimer as a Fluorescence Probe for Protein Assays

Abstract

A spectrofluorometric method was developed for the determination of total serum protein by exploring toluidine blue (TB) as the fluorescence probe. The fluorescence intensity of TB at 648 nm was significantly quenched in the presence of sodium dodecylbenzene sulfonate (SDBS) by forming a dimer of the dye, which can afterwards reconvert to monomer when proteins were added accompanied by the recovery of the fluorescence. This might be attributed to the modulated transferring of the dimer‐monomer equilibrium of TB in the anionic surfactant caused by the addition of protein. A linear calibration graph was obtained in the range of 0.5–50 mg/l BSA, with a detection limit of 0.15 mg/l and a RSD of 1.3% (n=11, 5.0 mg/l BSA). Total proteins in human serums were analyzed by using the present procedure and the results agreed well with those obtained by the Biuret method.     

Adsorptive immobilization of intestinal brush border membrane on triton X-100-substituted sepharose 4B

Triton X-100-substituted Sepharose 4B (Sepharose-TX) was used for adsorptive immobilization of intestinal brush border membrane using lactose-phlorizin hydrolase as a representative membrane enzyme. Limited heating of membrane preparations was found to enhance binding. This enhancement is concluded to be owing to a greater availability of the hydrophobic sites, as also confirmed by the 1-anilino-8-naphthalene sulfonate fluorescence studies, for interaction with Triton X-100 moieties on the support. The immobilized preparations obtained by this procedure were found useful in hydrolysis of lactose, involving lactose-phlorizin hydrolase, in continuous operations. It is suggested that the approach may be of general utility for immobilization of biologic membranes by interaction of their extramembrane structures using supports with appropriate hydrophobic groups.     

1,2,5,6-Tetrakis(guanidino)-Naphthalenes: Electron Donors,Fluorescent Probes and Redox-Active Ligands

New redox-active 1,2,5,6-tetrakis(guanidino)-naphthalene compounds, isolable and storable in the neutral and deep-green dicationic redox states and oxidisable further in two one-electron steps to the tetracations, are reported. Protonation switches on blue fluorescence, with the fluorescence intensity (quantum yield) increasing with the degree of protonation. Reactions with N-halogenosuccinimides or N-halogenophthalimides led to a series of new redox-active halogeno- and succinimido-/phthalimido-substituted derivatives. These highly selective reactions are proposed to proceed via the tri- or tetracationic state as the intermediate. The derivatives are oxidised reversibly at slightly higher potentials than that of the unsubstituted compounds to dications and further to tri- and tetracations. The integration of redox-active ligands in the transition-metal complexes shifts the redox potentials to higher values and also allows reversible oxidation in two potentially separated one-electron steps.     

Synthesis and characterization of azo-linked Schiff bases and their nickel(II), copper(II), and zinc(II) complexes

Azo compounds were prepared by coupling of benzenediazonium chloride ions with 1-amino-2-hydroxy-4-naphthalene sulfonic acid under alkaline conditions, and Schiff bases, L_1–3 were then obtained by the condensation of 1-amino-2-hydroxy-3-(phenylazo)-4-naphthalene sulfonic acid, 1-amino-2-hydroxy-3-(4-ethylphenylazo)-4-naphthalene sulfonic acid, and 1-amino-2-hydroxy-3-(4-nitrophenylazo)-4-naphthalene sulfonic acid with salicylaldehyde. New copper(II), nickel(II), and zinc(II) complexes of the Schiff base ligands were also prepared and characterized by spectroscopic methods, magnetic measurements, elemental, and thermogravimetric analysis.     

两种新型吡啶盐的合成，表征及双光子性质研究

本文报道了两种新的吡啶盐的合成，用元素分析、红外光谱、单晶X-射线衍射进行了表征。研究了它们的紫外光谱、荧光光谱和光限幅特性，发现它们的DMF溶液对1 064 nm皮秒脉冲激光表现出明显的光限幅特性。     

Determination of oroxylin A,oroxylin A 7‐O‐glucuronide,and oroxylin A sodium sulfonate in beagle dogs by using UHPLC MS/MS Application in a pharmacokinetic study

Oroxylin A, obtained from the root of Scutellaria baicalensis Georgi, is a flavonoid with antitumor and other pharmacological activities. Our previous studies showed for the first time that it is mainly metabolized to oroxylin A sodium sulfonate by sulfotransferase enzymes in beagle dogs. In this study, rapid, universal, selective, and robust ultra‐high‐performance liquid chromatography–tandem mass spectrometry methods were established and fully validated to quantitatively detect oroxylin A, oroxylin A 7‐O‐glucuronide, and oroxylin A sodium sulfonate in beagle dog plasma. The quantitative analysis for oroxylin A sodium sulfonate was reported for the first time. Plasma samples were processed with acetonitrile, a universal protein precipitant. Gradient elution was performed to resolve carryover effects and to achieve separation efficiency and sufficient chromatographic retention. The linear relationships of oroxylin A, oroxylin A 7‐O‐glucuronide, and oroxylin A sodium sulfonate in plasma were in the range of 2.0–500.0, 5.0–500.0, and 1.881–940.5 ng/mL, respectively. The assay method was successfully applied to pharmacokinetic study. This is the first paper that reveals the pharmacokinetic profile of oroxylin A, oroxylin A 7‐O‐glucuronide, and oroxylin A sodium sulfonate after single‐dose intravenous and oral administration of Oroxylin A in beagle dogs.     

Monitoring the Tanford transition in β‐lactoglobulin by 8‐anilino‐1‐naphthalene sulfonate and mass spectrometry

The fluorescent dye 8‐anilino‐1‐naphthalene sulfonate (ANS) is known to interact with proteins by conformation‐specific hydrophobic interactions and rather nonspecific electrostatic interactions. To which category the complexes detectable by mass spectrometry (MS) belong is still the subject of debate. Here, the Tanford transition in β‐lactoglobulin (BLG) is exploited as an experimental device to expose hydrophobic binding sites by an increase in pH, rather than, as usually done, by lowering the pH. Complex formation is monitored by electrospray ionization (ESI)‐MS and fluorescence spectroscopy. Both techniques reveal stronger ANS binding to BLG at pH 7.9 than at pH 5.9, suggesting that dye binding inside the calyx, which is known to be hydrophobically driven in solution, can contribute to the complexes detected by ESI‐MS. Electrostatic interactions between the protein and the ANS sulfonate group can only be weaker at pH 7.9 than at pH 5.9, supporting the interpretation of the results by the protein conformational change. Lysozyme is used as a negative control, which shows no variation in the interaction with ANS in the same range of pH, in the absence of conformational changes. However, comparison of MS and fluorescence data at variable pH for BLG and myoglobin (Mb) suggests that conformation‐specific ANS binding to proteins is detectable by ESI‐MS only inside well‐structured cavities of folded structures, like the BLG calyx and apoMb heme pocket. Indeed, ANS interactions with highly dynamic structures or molten globules, although detectable in solution, are easily lost in the gas phase. Copyright © 2008 John Wiley & Sons, Ltd.     

Dienol-Benzol-Umlagerung von Penta-2,4-dienyl-benzocyclohexadienolen

1-Hydroxy-2-methyl-2-(penta-2,4-dienyl)-1,2-dihydronaphthalene ( 2 ), on treatment with 0,75N H₂SO₄ in ether at 0°, underwent a [1s, 2s]-sigmatropic rearrangement to give 2-methyl-1-(penta-2,4-dienyl)-naphthalene ( 5 ), cf. scheme 2. 2-Hydroxy-1-methyl-1-(penta-2,4-dienyl)-1,2-dihydronaphthalene ( 4 ) under the same conditions gave 38% of the [1s, 2s]-product 1-methyl-2-(penta-2,4-dienyl)-naphthalene ( 6 ), together with 26% 1-methylnaphthalene, 21% 1-methyl-4-(penta-2,4-dienyl)-naphthalene ( 7 ) and 1% 1-methyl-5-(penta-2,4-dienyl)-naphthalene ( 8 ), cf. scheme 2. Most likely the latter two naphthalene derivatives at least are products of an intermolecular process.     

Chromatographic Separation and Mass Spectrometric Analysis of Bacterial Cell Wall Synthesizing Enzyme Complexes

ABSTRACT

Penicillin-binding proteins (PBPs) were shown to associate non-covalently with many other morphogene proteins (MGPs). Specific associations were assigned. The PBPs were labeled with spectroscopic/fluorescence (F/S) groups in the form of dansylated β-lactam probes. Competitive β-lactam binding of non-denatured PBP/MGP complexes led to characteristic patterns of F/S labeling by the probes. The salt-bridge specific reagent, ethanedinitrile, covalently linked various MGPs to the F/S labeled PBPs. Proteolysis of chromatographically purified F/S labeled fractions gave sets of peptides analyzed by MALDI-TOF to give MH data. Peptide mass-fingerprinting analysis revealed that covalent linkage occurred with other MGPs and not with non-MGP proteins of ～3400 proteins in the SWISS-PROT r33 data base for E. coli K-12.     

A chromatographic estimate of the degree of surface heterogeneity of RPLC packing materials. III. Endcapped amido-embedded reversed phase

The difference in adsorption behavior between a conventional monomeric endcapped C18 stationary phase (3.43 micromol/m2) and an endcapped polymeric RP-Amide phase (3.31 micromol/m2) was investigated. The adsorption isotherms of four compounds (phenol, caffeine, sodium 2-naphthalene sulfonate, and propranololium chloride) were measured by frontal analysis (FA) and the degree of heterogeneity of each phase for each solute was characterized by their adsorption energy distributions (AED), derived using the Expectation-Maximization method. The results show that only certain analytes (phenol and 2-naphthalene sulfonate) are sensitive to the presence of the polar embedded amide groups within the RP phase. Their binding constants on the amide-bonded phase are significantly higher than on conventional RPLC phases. Furthermore, an additional type of adsorption sites was observed for these two compounds. However, these sites having a low density, their presence does not affect much the retention factors of the two analytes. On the other hand, the adsorption behavior of the other two analytes (caffeine and propranololium chloride) is almost unaffected by the presence of the amide group in the bonded layer. Strong selective interactions may explain these observations. For example, hydrogen-bond interactions between an analyte (e.g., phenol or naphthalene sulfonate) and the carbonyl group (acceptor) or the nitrogen (donor) of the amido-embedded group may take place. No such interactions may take place with either caffeine or the cation propranololium chloride. This study confirms the hypothesis that analytes have ready access to locations deep inside the bonded layer, where the amide groups are present.     

Protein–induced aggregation of fluorescent conjugated polyelectrolytes with sulfonate groups: Synthesis and its sensing application

Anionically charged fluorescent conjugated polyelectrolytes of poly{[4,7‐(2,1,3‐benzothiadiazole)‐alt‐1,4‐phenylene]‐co‐[2,5‐bis(4‐sulfonatobutoxy)‐alt‐1,4‐phenylene]} ( P1 ) and poly{[4,7‐(bis(thiophen‐2‐yl)benzo‐2,1,3‐thiadiazole)‐alt‐1,4‐phenylene]‐co‐[2,5‐bis(4‐sulfonatobutoxy)‐alt‐1,4‐phenylene]} ( P2 ) were synthesized by Suzuki crosscoupling polymerization in the presence of a palladium catalyst. The conjugated polyelectrolytes with sulfonate groups, as efficient signal amplifying reporters, were carefully designed to be soluble in water over the entire pH range examined and interact with proteins through intermolecular forces. The polymers exhibited blue emission in aqueous solutions but green or red emission in solid form depending on the conjugation length due to intermolecular exciton migration. The anionic conjugated polymers exhibited blue‐to‐green or blue‐to‐red changes in fluorescence upon exposure to charged proteins, indicating that the polymers have potential applications in fluorescent array systems for protein. © 2010 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem, 2010