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Electrospray Mass Spectrometry (electrospray + mass_spectrometry)
Selected AbstractsStructure-Dependent Electrochemical Behavior of Thienylplatinum(II) Complexes of N,N-HeterocyclesEUROPEAN JOURNAL OF INORGANIC CHEMISTRY, Issue 1 2004Feng Zhao Abstract trans -[Pt(MeCN)(PPh3)2(2-thienyl)]BF4 (1) serves as a convenient precursor to bifunctional mononuclear trans -[Pt(PPh3)2(,1 - N - N)(2-thienyl)]BF4 [N - N = pyrazine (2); 2-chloropyrazine, (3)] and dinuclear trans,trans -[Pt2(PPh3)4(,- N - N)(2-thienyl)2](BF4)2 [(N - N = 4,4, -bipyridine (4); 4,4, -vinylenedipyridine (5)] complexes. The nuclear selectivity is conveniently controlled by the choice of the heterocyclic ligands or spacers. Both structural types 3 and 5 were confirmed by single-crystal X-ray crystallographic analyses. Their solution identities were established by positive-ion Electrospray Mass Spectrometry (ESMS). The electroactivities of these complexes were studied by cyclic voltammetry (CV). Continuous CV scans of 4 and 5 revealed variations in the redox waves with the number of scans. While the initial oxidative scan exhibited only a broad, irreversible wave, further cycling showed the growth of two additional redox couples up to about the tenth cycle. The peak currents of these redox couples began to decay with prolonged potential cycling beyond the tenth cycle. These findings are consistent with the formation of electroactive oligomers/polymers, and this conclusion is supported by visible thin film formation on the electrodes. In contrast, the mononuclear complexes (2 and 3) do not show such behavior. The films formed were further studied by repetitive potential cycling and XPS. (© Wiley-VCH Verlag GmbH & Co. KGaA, 69451 Weinheim, Germany, 2004) [source] Monitoring the Formation of Coordination Complexes Using Electrospray Mass SpectrometryCHEMISTRY - AN ASIAN JOURNAL, Issue 5 2009Jennifer Abstract Linked-in: The rigid Schiff-base ligand cis,trans -1,3,5-tris(pyridine-2-carboxaldimino) cyclohexane (ttop) is synthesized, and its complexation to copper(II) salts at a range of stoichiometries is investigated crystallographically by using electrospray mass spectrometry. Further, in-situ mass spectrometry measurements allow the stepwise construction of the complexes to be observed. cis,trans -1,3,5-Triaminocyclohexane (trans -tach) has been shown to be an excellent ligand in the synthesis of discrete complexes, molecular clusters, and infinite architectures. Herein, we report the Schiff-base derivitization of trans -tach to form cis,trans -1,3,5- tris (pyridine-2-carboxaldimino) cyclohexane (ttop), and the complexation of this ligand with copper(II) salts. The complexation reaction leads to the crystallization of transition-metal complexes with nuclearities of 1, 2, and 4, and the formation of the complexes can be followed stepwise, in real time, using electrospray mass spectrometry. [source] Study on the Gas Phase Stability of Heme-binding Pocket in Cytochrome Tb5 and Its Mutants by Electrospray Mass SpectrometryCHINESE JOURNAL OF CHEMISTRY, Issue 12 2002Chong-Tian Yu Abstract To elucidate the effect of various amino add residues on the heme-binding pocket in cytochrome Tb5, several residues were chosen for replacement by means of site-directed mutagenesis. Comparison of the mass spectrum between the F35Y mutant and the wild type shows that the relative abundance of holoprotein ion of F35Y is lower than that of the wild type in gas phase. It is concluded that mutation from Phe35 residue to tyrosine decreases the hydrophobic character of cytochrome Tb5 heme pocket, which decreases the stability of heme-binding pocket. ESI-MS spectra of the mutants V61E, V61K, V61H and V61Y show various contribution of amino acid to the stability of heme-binding pocket. The small and non-polar residue Val61 was replaced with large or polar residues, resulting in enhancing the trend of heme leaving from the pocket. In addition, comparison of the mass relative abundance of holo-proteins among all the Vakil-mutants, shows mat their stability in gas phase appropriately submit the following order: wild type > V61H > V61E > V61K , V61Y. The extra great stability of quadruple sites mutant E44/48/56A/D60A shows that reduction of electrostatic or hydrogen bond interactions among the residues locating in the outside region of the heme edge remarkably affect the stability of heme. The results of analyzing the oxidation states of heme iron in Tb5 and its mutants by insource-CAD experiment suggest that the charge states of heme iron Maintain inflexible in mutation process. [source] Electrospray mass spectrometry of stable iminyl nitroxide and nitronyl nitroxide free radicalsJOURNAL OF MASS SPECTROMETRY (INCORP BIOLOGICAL MASS SPECTROMETRY), Issue 9 2002Craig D. Smith Abstract Electrospray ionization (ESI) mass spectra have been recorded for a range of substituted nitronyl nitroxide and iminyl nitroxide monoradicals and biradicals. Secondary species formed in the ESI source were observed as the dominant ions in both the iminyl nitroxide and nitronyl nitroxide spectra. Daughter ion spectrometry was used to establish fragmentation mechanisms for the nitronyl nitroxide and iminyl nitroxide moieties as well as the secondary species under ESI conditions. Copyright © 2002 John Wiley & Sons, Ltd. [source] Physicochemical consequences of the perdeuteriation of glutathione S -transferase from S. japonicumPROTEIN SCIENCE, Issue 3 2001David Brockwell Abstract Glutathione S -transferase (GST) from Schistosoma japonicum has been prepared in both normal protiated (pGST) and fully deuteriated (dGST) form by recombinant DNA technology. Electrospray mass spectrometry showed that the level of deuteriation in dGST was 96% and was homogeneous across the sample. This result is attributed to the use of a deuterium-tolerant host Escherichia coli strain in the preparation of the protein. 10 heteroatom-bound deuteriums (in addition to the carbon-bound deuteriums) were resistant to exchange when dGST was incubated in protiated buffer. The physicochemical and biological properties of the two proteins were compared. dGST was relatively less stable to heat denaturation and to proteolytic cleavage than was pGST. The midpoint transition temperature for pGST was 54.9°C, whereas that for dGST was 51.0°C. Static light-scattering measurements revealed that the association behavior of dGST is also different from that of pGST. The perdeuteriated enzyme shows a tendency to associate into dimers of the fundamental dimer. This is in contrast with results that have been obtained for other perdeuteriated proteins in which perdeuteriation has been shown to promote dissociation of aggregates. dGST showed a similar Km to pGST; similar results had been obtained previously with bacterial alkaline phosphatase. However, whereas the alkaline phosphatase showed a reduced rate of catalysis on deuteriation, dGST exhibited a slightly higher rate of catalysis than pGST. It is clear that the bulk substitution of deuterium for protium has significant effects on the properties of proteins. Until many more examples have been studied, it will be difficult to predict these effects for any given protein. Nevertheless, deuteriation represents an intriguing method of preparing functional analogs of recombinant proteins. [source] Studies of phospholipid oxidation by electrospray mass spectrometry: From analysis in cells to biological effectsBIOFACTORS, Issue 1-4 2005Corinne M. Spickett Abstract The oxidation of lipids is important in many pathological conditions and lipid peroxidation products such as 4-hydroxynonenal (HNE) and other aldehydes are commonly measured as biomarkers of oxidative stress. However, it is often useful to complement this with analysis of the original oxidized phospholipid. Electrospray mass spectrometry (ESMS) provides an informative method for detecting oxidative alterations to phospholipids, and has been used to investigate oxidative damage to cells, and low-density lipoprotein, as well as for the analysis of oxidized phosphatidylcholines present in atherosclerotic plaque material. There is increasing evidence that intact oxidized phospholipids have biological effects; in particular, oxidation products of 1-palmitoyl-2-arachidonoyl- sn -glycerophosphocholine (PAPC) have been found to cause inflammatory responses, which could be potentially important in the progression of atherosclerosis. The effects of chlorohydrin derivatives of lipids have been much less studied, but it is clear that free fatty acid chlorohydrins and phosphatidylcholine chlorohydrins are toxic to cells at concentrations above 10 micromolar, a range comparable to that of HNE and oxidized PAPC. There is some evidence that chlorohydrins have biological effects that may be relevant to atherosclerosis, but further work is needed to elucidate their pro-inflammatory properties, and to understand the mechanisms and balance of biological effects that could result from oxidation of complex mixtures of lipids in a pathophysiological situation. [source] Synthesis and Structural Characterisation of Copper(II) 15-Metallacrown-5 Complexes with PbII, HgII, AgI, NaI and YIII Central Metal IonsEUROPEAN JOURNAL OF INORGANIC CHEMISTRY, Issue 19 2007Sabry Hamed Seda Abstract The new copper(II) 15-metallacrown-5 complexes with the central metal ions PbII, HgII, AgI, NaI and YIII, with the formula [MCu5L5]Xn {H2L is 2-picolinehydroxamic acid or (S)-phenylalaninehydroxamic acid and X, is NO3, or Cl,}, have been synthesised and characterised by NMR and UV/Vis spectroscopy, electrospray mass spectrometry and elemental analysis. The PbII - and HgII 15-metallacrown-5 complexes were obtained in the crystalline form as pyridine adducts [PbCu5(picha)5(py)6](NO3)2·3(py) and [HgCu5(picha)5(py)7](NO3)2·2(py) and their X-ray crystal structures were determined. In both complexes, each peripheral CuII ion of the metallacrown is coordinated by one pyridine molecule bonded in the axial position. In the case of the PbII derivative, one additional axial pyridine molecule is bound to the central metal ion, while in the case of the HgII derivative, two axial pyridine ligands are bound to the central HgII ion. The relative stability of the copper(II) 15-metallacrown-5 complexes with various central metal ions was determined on the basis of competition reactions. The relative preference of the 15-metallacrown-5 system for the central metal ion follows the series NaI, AgI < lanthanide(III), HgII < PbII.(© Wiley-VCH Verlag GmbH & Co. KGaA, 69451 Weinheim, Germany, 2007) [source] Dimeric 2,2,-Bipyridylruthenium(II) Complexes Containing 2,2,-Bis(1,2,4-triazin-3-yl)-4,4,-bipyridine-Like Bridging Ligands: Syntheses, Characterization and DNA BindingEUROPEAN JOURNAL OF INORGANIC CHEMISTRY, Issue 11 2004Cai-Wu Jiang Abstract Three new bridging ligands 2,2,-bis(1,2,4-triazin-3-yl)-4,4,-bipyridine (btb), 2,2,-bis(1,2,4-triazino[5,6-f]acenaphthylen-3-yl)-4,4,-bipyridine (btapb), 2,2,-bis(5,6-diphenyl-1,2,4-triazin-3-yl)-4,4,-bipyridine (bdptb) and their dimeric 2,2,-bipyridylruthenium(II) complexes [Ru(bpy)2(btb)Ru(bpy)2]4+ (1), [Ru(bpy)2(btapb)Ru(bpy)2]4+ (2), [Ru(bpy)2(bdptb)Ru(bpy)2]4+ (3) have been synthesized and characterized by elemental analysis, fast atom bombardment (FAB) mass spectrometry or electrospray mass spectrometry (ES-MS), 1H NMR and UV/Visible spectroscopy. The binding behavior of these dimeric complexes with calf thymus DNA (CT-DNA) was investigated by electronic absorption spectroscopy, viscosity measurements, and equilibrium dialysis experiments. The hypochromism of the metal-ligand charge transfer (MLCT) band in the electronic absorption spectra of the dinuclear complexes 1, 2, and 3 is 8.7%, 19% and 33%, respectively, with bathochromic shifts of 5, 5 and 14 nm, respectively. The binding constants are 7.5×104M,1, 4.8×105M,1 and 7.6×105M,1, respectively. Increasing the size of the plane of the bridging ligand increases the hydrophobicity of their complexes, leading to stronger binding by the complexes to calf thymus DNA. The effect of increasing concentrations of these novel dimeric ruthenium(II) complexes on the relative viscosities of CT-DNA is less notable than that of well-known intercalators such as [Ru(bpy)2(dppz)]2+. The equilibrium experiments showed that ,,,3 binding is stronger than ,,,3 binding to CT-DNA. This is the first example of a dinuclear complex binding enantioselectively to CT-DNA measured by equilibrium dialysis. The experiments suggest that the three complexes may be DNA groove binders. (© Wiley-VCH Verlag GmbH & Co. KGaA, 69451 Weinheim, Germany, 2004) [source] Inactivation of Aeromonas hydrophila metallo-,-lactamase by cephamycins and moxalactamFEBS JOURNAL, Issue 13 2001Astrid Zervosen Incubation of moxalactam and cefoxitin with the Aeromonas hydrophila metallo-,-lactamase CphA leads to enzyme-catalyzed hydrolysis of both compounds and to irreversible inactivation of the enzyme by the reaction products. As shown by electrospray mass spectrometry, the inactivation of CphA by cefoxitin and moxalactam is accompanied by the formation of stable adducts with mass increases of 445 and 111 Da, respectively. The single thiol group of the inactivated enzyme is no longer titrable, and dithiothreitol treatment of the complexes partially restores the catalytic activity. The mechanism of inactivation by moxalactam was studied in detail. Hydrolysis of moxalactam is followed by elimination of the 3, leaving group (5-mercapto-1-methyltetrazole), which forms a disulfide bond with the cysteine residue of CphA located in the active site. Interestingly, this reaction is catalyzed by cacodylate. [source] Design, synthesis and properties of synthetic chlorophyll proteinsFEBS JOURNAL, Issue 11 2001Harald K. Rau A chemoselective method is described for coupling chlorophyll derivatives with an aldehyde group to synthetic peptides or proteins modified with an aminoxyacetyl group at the ,-amino group of a lysine residue. Three template-assembled antiparallel four-helix bundles were synthesized for the ligation of one or two chlorophylls. This was achieved by coupling unprotected peptides to cysteine residues of a cyclic decapeptide by thioether formation. The amphiphilic helices were designed to form a hydrophobic pocket for the chlorophyll derivatives. Chlorophyll derivatives Zn-methylpheophorbide b and Zn-methyl-pyropheophorbide d were used. The aldehyde group of these chlorophyll derivatives was ligated to the modified lysine group to form an oxime bond. The peptide,chlorophyll conjugates were characterized by electrospray mass spectrometry, analytical HPLC, and UV/visible spectroscopy. Two four-helix bundle chlorophyll conjugates were further characterized by size-exclusion chromatography, circular dichroism, and resonance Raman spectroscopy. [source] Differences in the skin peptides of the male and female Australian tree frog Litoria splendidaFEBS JOURNAL, Issue 1 2000The discovery of the aquatic male sex pheromone splendipherin, a new antibiotic peptide caerin 1.10, together with Phe8 caerulein The skin secretions of female and male Litoria splendida have been monitored monthly over a three-year period using HPLC and electrospray mass spectrometry. Two minor peptides are present only in the skin secretion of the male. The first of these is the female-attracting aquatic male sex pheromone that we have named splendipherin, a 25 amino acid peptide (GLVSSIGKALGGLLADVVKSKGQPA-OH). This pheromone constitutes about 1% of the total skin peptides during the breeding season (January to March), dropping to about 0.1% during the period June to November. Splendipherin attracts the female in water at a concentration of 10,11,10,9 m, and is species specific. The second peptide is a wide-spectrum antibiotic of the caerin 1 group, a 25 residue peptide (GLLSVLGSVAKHVLPHVVPVIAEKL-NH2) named caerin 1.10. The neuropeptides of L. splendida are also seasonally variable, the change identical for both the female and male. During the period October to March, the sole neuropeptide present in skin secretions is caerulein [pEQDY(SO3)TGWMDF-NH2]; this is active on smooth muscle and is also an analgaesic. During the southern winter (June to September), more than half of the caerulein is hydrolysed to [pEQDYTGWMDF-NH2], a peptide that shows no smooth muscle activity. In place of caerulein, a new peptide, Phe8 caerulein [pEQDY(SO3)TGWFDF-NH2], becomes a major component of the skin secretion. Perhaps this seasonal change is involved in thermoregulation, that is, with the initiation and maintenance of the inactive (hibernation) phase of the animal. [source] Tetrabutylammonium salt of the B24F224, anion.HETEROATOM CHEMISTRY, Issue 3 20062e BB bond, Two B12F11, icosahedra linked by a 2c, surrounded by a sheath of CH· · ·FB hydrogen bonds The B24F224, anion, which was formed as a minor by-product when the B12H122, anion was treated with F2 in liquid HF, has been isolated as its N(n-Bu)4+ salt and characterized by 10B, 11B, and 19F NMR spectroscopy, electrospray mass spectrometry, cyclic voltammetry, single-crystal X-ray diffraction, and calculations at the DFT level of theory. The B24F224, anion has idealized D5 symmetry and consists of two B12F112, icosahedra linked by a 2c,2e boron,boron single bond with a BB distance of 1.725(4) Å. In the solid state, the anion interacts with eight N(n-Bu)4+ cations via a network of 34 CH···FB hydrogen bonds with H· · ·F distances that range from 2.26 to 2.55 Å. These hydrogen bonds were successfully modeled by DFT calculations, which showed that the hydrogen bonds probably have a measurable, albeit subtle, effect on the structure of the B24F224,. © 2006 Wiley Periodicals, Inc. Heteroatom Chem 17:181,187, 2006; Published online in Wiley InterScience (www.interscience.wiley.com). DOI 10.1002/hc.20220 [source] Microwave-assisted nucleophilic cleavage of 5,7-dimethyl-2-phenyl-1-oxo-lH -pyrazolo[ 1,2- a]pyrazol-4-ylium-3-olate to ,-phenylmalonamidesJOURNAL OF HETEROCYCLIC CHEMISTRY, Issue 7 2005Daniel E. Lynch Three ,-phenylmalonamides have been prepared by the selective nucleophilic cleavage of 5,7-dimethyl-2-phenyl-1-oxo-1H -pyrazolo[1,2- a]pyrazol-4-ylium-3-olate in solventless microwave syntheses. The three weak nucleophiles employed were aniline, p -chloroaniline and m -toluidine. The ,-phenylmalonamides of these three aniline derivatives could not be prepared using the previously reported solvent syntheses via 3-oxopyrazolo[1,2- a]pyrazol-8-ylium-1-olates. All products were characterised using, infrared spectroscopy, 1H nmr and electrospray mass spectrometry. The single crystal X-ray structures of the starting pyrazolo-[1,2- a]pyrazole and ,-phenylmalon- m -toluidide are also reported. [source] Metabolomic fingerprinting of plant extracts,JOURNAL OF MASS SPECTROMETRY (INCORP BIOLOGICAL MASS SPECTROMETRY), Issue 12 2006L. Mattoli Abstract The standardization and quality control of plant extracts is an important topic, in particular, when such extracts are used for medicinal purposes. Consequently, the development of fast and effective analytical methods for metabolomic fingerprinting of plant extracts is of high interest. In this investigation, electrospray mass spectrometry (ESI-MS) and 1H NMR techniques were employed with further statistical analyses of the acquired data. The results showed that negative ion mode ESI-MS is particularly effective for characterization of plant extracts. Different samples of the same species appear well-clustered and separated from the other species. To verify the effectiveness of the method, two other batches of extracts from a species, in which the principal components were already identified (Cynara scolymus), were analyzed, and the components that were verified by the principal component analysis (PCA) were found to be within the region identified as characteristic of Cynara Scolymus extracts. The data from extracts of the other species were well separated from those pertaining to the species previously characterized. Only the case of a species that was strictly correlated from a botanical point of view, with extracts that were previously analyzed, showed overlapping. Copyright © 2006 John Wiley & Sons, Ltd. [source] Improved protonation, collision-induced decomposition efficiency and structural assessment for ,red tide' brevetoxins employing nanoelectrospray mass spectrometryJOURNAL OF MASS SPECTROMETRY (INCORP BIOLOGICAL MASS SPECTROMETRY), Issue 8 2006Weiqun Wang Abstract Brevetoxins are a group of natural neurotoxins found in blooms of red tide algae. Previous electrospray mass spectrometry (ES-MS) studies show that all brevetoxins have high affinities for sodium ions, and they form abundant sodium adduct ions, [M + Na]+, in ES-MS, even when trace contamination is the only source of sodium ions. Attempts to obtain informative product ions from the collision-induced decomposition (CID) of [M + Na]+ brevetoxin precursor ions resulted only in uninformative sodium ion signals, even under elevated collision energies. In this study, a nano-ES-MS approach was developed wherein ammonium fluoride was used to form cationic [M + NH4]+ adducts of brevetoxin-2 and brevetoxin-3; a significant increase in the abundance of protonated brevetoxin molecules [M + H]+ also resulted, whereas the abundance of sodium adducts of brevetoxins [M + Na]+ was observed to decrease. Under CID, both [M + NH4]+ and [M + H]+ gave similar, abundant product ions and thus underwent the same types of fragmentation. This indicated that ammonium ions initially attached to brevetoxins forming [M + NH4]+ easily lose neutral ammonia in a first step in the gas phase, leaving protonated brevetoxin [M + H]+ to readily undergo further fragmentation under CID. Copyright © 2006 John Wiley & Sons, Ltd. [source] Hydrolysis of the amyloid ,-peptide (A,) 1,40 between Asp23,Val24 produces non-aggregating fragments.JOURNAL OF MASS SPECTROMETRY (INCORP BIOLOGICAL MASS SPECTROMETRY), Issue 2 2005An electrospray mass spectrometric study Abstract The aggregation of full-length (residues 1,40) amyloid ,-peptide (A,) and fragments corresponding to residues 1,23 and 24,40 was studied by electrospray mass spectrometry, using gramicidin as a non-aggregating reference. Following a lag period, A,(1,40) at 140 µM concentration aggregates with apparent first-order kinetics. Under acidic conditions A,(1,40) undergoes spontaneous cleavage between Asp23,Val24 and to a lesser extent also at two other Asp,X motifs. Incubation in acidic H218O showed incorporation of 18O in fragment A,(1,23), confirming that the Asp23,Val24 peptide bond had been hydrolyzed. Incubation of synthetic A,(1,23) and A,(24,40) peptides with A,(1,40) showed that A,(24,40) remained in solution for several months, that A,(1,23) partly disappeared from solution, whereas A,(1,40) completely disappeared. Further, treatment of sedimentable aggregates formed after co-incubation of the three peptides with hexafluoro-2-propanol or formic acid recovered the intensity of A,(1,40). These data support previous studies showing that the region of A, encompassing residues 16,24 is necessary for aggregation into amyloid fibrils. Copyright © 2005 John Wiley & Sons, Ltd. [source] Qualitative study of in vivo melphalan adduct formation in the rat by miniaturized column-switching liquid chromatography coupled with electrospray mass spectrometryJOURNAL OF MASS SPECTROMETRY (INCORP BIOLOGICAL MASS SPECTROMETRY), Issue 1 2004Bart Van den Driessche Abstract In a general study of DNA adduct formation with melphalan, rats were intravenously injected with a single high dose (10 mg kg,1). Adduct formation was studied at the nucleoside level in the target organs liver, bone marrow, kidney and blood with the use of 2D liquid chromatography/tandem mass spectrometry (LC/MS/MS). Adducts of dGuo and dAdo were detected under selected reaction monitoring in liver and bone marrow 10 h after administration of melphalan. In the DNA hydrolysates from kidney and blood a Gua,melphalan adduct was found, although in very low abundance. These first results of the search for in vivo -formed melphalan adducts in the rat showed that our miniaturized LC/MS technique is useful for investigating this type of compound. More experiments will be performed in this area to gather more information about the pharmacokinetics and the quantity of adducts formed. Copyright © 2003 John Wiley & Sons, Ltd. [source] Increased vigabatrin entry into the brain by polysorbate 80 and sodium caprateJOURNAL OF PHARMACY AND PHARMACOLOGY: AN INTERNATI ONAL JOURNAL OF PHARMACEUTICAL SCIENCE, Issue 2 2001D. Dimitrijevic The effects of a non-ionic surfactant, polysorbate 80, and the sodium salt of the saturated fatty acid, sodium caprate (C10), as potential brain absorption enhancers for vigabatrin were studied. Vigabatrin is an enzyme-activated irreversible inhibitor of ,-aminobutyric acid (GABA) transaminase that increases brain and cerebrospinal GABA concentrations in animals and man. Before intravenous administration, a range of concentrations of the surfactants were tested using erythrocyte lysis or the red blood cell lysis test to establish the non-toxic concentration range. Vigabatrin was dissolved in 0.1% polysorbate 80 and 0.1% sodium caprate and administered intravenously in doses of 4 mL kg,1 to male Wistar rats (230,250 g; n = 3). Rats were killed 2 h after drug and surfactant administration and the brains were immediately removed and homogenized in 0.4m perchloric acid. Selected ion monitoring electrospray mass spectrometry was used to determine the concentration of vigabatrin and GABA directly from the perchloric acid extract of the rat brain. This method was developed to increase the speed and efficiency of the analysis by removing the need for complex extraction and derivatization procedures while retaining the specificity of the mass spectrometer as a detector. The stability of both vigabatrin and GABA in perchloric acid was established by monitoring their pseudo molecular ions in standard solutions at timed intervals over 24 h. Although the detection level for vigabatrin and GABA was at least 50 pg, only GABA was detected in rat brain. Vigabatrin caused a small increase in whole brain GABA. However, GABA levels were higher in the samples with vigabatrin + enhancer than in the samples where vigabatrin alone was administered. One-way analysis of variance indicated a significant effect of the surfactants on GABA levels (F (5,17) = 11.86, P < 0.01) and vigabatrin absorption was presumed. The rectal temperature of the rats is lowered by the presence of vigabatrin in the brain. Vigabatrin alone decreased rectal temperature by 6%. When given with either polysorbate 80 or sodium caprate, the extent of temperature lowering was significantly greater (P < 0.001). There was no significant difference after 2 h between polysorbate 80 + vigabatrin, and sodium caprate + vigabatrin. [source] Synthesis and stability study of dental monomers containing methacrylamidoethyl phosphonic acidsJOURNAL OF POLYMER SCIENCE (IN TWO SECTIONS), Issue 1 2007Xiaoming Xu Abstract Three new dental monomers containing methacrylamidoethyl phosphonic acids were synthesized. The structures of the synthesized monomers were determined with electrospray mass spectrometry (ESMS), Fourier transform infrared, and NMR. The hydrolytic stabilities of the synthesized monomers and a commercial monomer, 2-methacryloyloxyethyl phosphoric acid (MEP; used as a control), were studied with flow injection (FI)/ESMS, 1H NMR, and 31P NMR analysis of a CD3OD/D2O (4:1 v/v) solution of each monomer before and after storage at 60 °C for 2 months. The 1H NMR and 31P NMR chemical shifts of the monomers 2-methacrylamidoethylphosphonic acid (I) and N,N,-[4,4,-(propane-2,2-diyl)-bis(phenoxy-2-hydroxypropyl)]-bis(2-methacrylamidoethylphosphonic acid) (II) showed little change after storage at 60 °C for 2 months, but those of MEP changed significantly. FI/ESMS also showed that MEP was nearly completely decomposed, whereas monomers I and II remained largely intact. MEP could react with H2ZrF6 to form ternary zirconium fluoride complexes that were partially soluble in methanol, but all the monomers containing phosphonic acids formed precipitates. This study demonstrates that ESMS is a more sensitive and effective method than NMR for studying the hydrolytic stability or degradation of dental monomers. The new monomers containing methacrylamidoethyl phosphonic acids have higher hydrolytic stability than methacrylate phosphate monomers and may be used in dental bonding agents and other dental materials. © 2006 Wiley Periodicals, Inc. J Polym Sci Part A: Polym Chem 45: 99,110, 2007 [source] Simultaneous determination of melamine and related compounds by hydrophilic interaction liquid chromatography,electrospray mass spectrometryJOURNAL OF SEPARATION SCIENCE, JSS, Issue 17-18 2010Jingen Xia Abstract A hydrophilic interaction liquid chromatography coupled to ESI-MS (HILIC/ESI-MS) method for the simultaneous determination of melamine and related compounds, i.e. ammeline, ammelide and cyanuric acid in foods was developed and validated. The separation was accomplished on a Venusil HILIC column with a mobile phase of acetonitrile + 10,mM ammonium formate buffer solution at pH 3.5 (88:12, v/v) under isocratic elution mode. For the detection of the targets, the ESI probe worked in the positive and negative switching mode. For each compound, three ions were selected as qualitative ions to obtain high specificity, and the most abundant ion of each compound was selected for quantification to obtain high sensitivity. The target compounds were quantified using SIM with 15N3-melamine and 13C3-cyanuric acid being used as an internal standards in the positive and negative modes, respectively. Compared with RP separation mode, HILIC has merits such as high separation and anti-interference efficiency. The method validation including linearity, LOD, LOQ, precision and recovery proved that the method has merits such high sensitivity, specificity and simplicity versus the other methods reported in the literature. [source] Copper-coated microsprayer interface for on-line sheathless capillary electrophoresis electrospray mass spectrometry of carbohydratesJOURNAL OF SEPARATION SCIENCE, JSS, Issue 3 2006Alina D. Zamfir Abstract A sturdy home-built sheathless CE/ESI-QTOF-MS system was developed and optimized for carbohydrate analysis. The interface and employed methodology provided a simple analytical solution to laborious CE/MS interfacing methods and to problems in characterization of complex carbohydrate mixtures that require high-resolution separation of the components. The CE/ESI interface, feasible in any MS laboratory, consists of a one-piece CE column having the CE terminus in-laboratory shaped as a microsprayer and coated with copper. The CE microsprayer was inserted into an in-house made stainless steel clenching device and the whole assembly was mounted onto a quadrupole TOF mass spectrometer. The analytical potential of the interface in terms of suitability, microsprayer performance, copper coat durability, ionization efficiency, spray stability, and sensitivity was tested first on a simple mixture of standard saccharides, which were separated, resolved, and detected with high separation efficiency. The approach was next assessed for the screening of a biological sample, a complex mixture of O -glycosylated sialylated amino acids from urine of a patient suffering from Schindler disease. Preliminary data allow this method to be considered as one of general applicability in structural glycobiology and glycomics and easy to be implemented for proteomic surveys as well. [source] Capillary columns in liquid chromatography: between conventional columns and microchipsJOURNAL OF SEPARATION SCIENCE, JSS, Issue 17-18 2004Yoshihiro Saito Abstract Liquid chromatography on columns with small internal diameters has been reviewed as the intermediate technique between conventional liquid chromatography and microchip separations. The development of micro column separations in the early years has been described, starting with the papers of Horváth and co-workers and Ishii and co-workers, continuing into the first part of the eighties, then making a leap in time to recent innovations with small-bore columns. Based on internal diameters a classification of the different analytical HPLC columns has been suggested. The advantages of small-bore columns have been discussed, with particular emphasis on the advantage of coupling to concentration sensitive detectors when the sample amount is limited. Open tubular columns are treated as a part of the historic background. The recent developments include a brief look into the current status of monolithic columns, the use of packed nano columns and micro columns with electrospray mass spectrometry, and the potential of two-dimensional comprehensive liquid chromatography. Finally, the coupling of sample preparation to analytical columns and the future applications of the novel technological improvements to the microchip separation methods have been discussed. [source] Detection of orange juice adulteration by tangelo juice using multivariate analysis of polymethoxylated flavones and carotenoidsJOURNAL OF THE SCIENCE OF FOOD AND AGRICULTURE, Issue 4 2002Geoffrey G Pan Abstract Reverse phase HPLC has been applied to quantify levels of polymethoxylated flavones and carotenoids in orange and tangelo juices. Lower levels of sinensetin and tetramethyl- o -scutellarein and higher levels of heptamethoxyflavone and tangeretin relative to nobiletin indicated the addition of tangelo to orange juice. ,-Cryptoxanthin and its esters, identified by positive ion electrospray mass spectrometry, were present in larger amounts relative to ,-carotene in tangelo than in orange juice. Using canonical discriminant analysis, the addition of 100,g,kg,1 tangelo to orange juice can be detected. © 2002 Society of Chemical Industry [source] Chip-mass spectrometry for glycomic studiesMASS SPECTROMETRY REVIEWS, Issue 2 2009Laura Bindila Abstract The introduction of micro- and nanochip front end technologies for electrospray mass spectrometry addressed a major challenge in carbohydrate analysis: high sensitivity structural determination and heterogeneity assessment in high dynamic range mixtures of biological origin. Chip-enhanced electrospray ionization was demonstrated to provide reproducible performance irrespective of the type of carbohydrate, while the amenability of chip systems for coupling with different mass spectrometers greatly advance the chip/MS technique as a versatile key tool in glycomic studies. A more accurate representation of the glycan repertoire to include novel biologically-relevant information was achieved in different biological sources, asserting this technique as a valuable tool in glycan biomarker discovery and monitoring. Additionally, the integration of various analytical functions onto chip devices and direct hyphenation to MS proved its potential for glycan analysis during the recent years, whereby a new analytical tool is on the verge of maturation: lab-on-chip MS glycomics. The achievements until early beginning of 2007 on the implementation of chip- and functional integrated chip/MS in systems glycobiology studies are reviewed here. © 2009 Wiley Periodicals, Inc., Mass Spec Rev 28:223,253, 2009 [source] Application of capillary electrophoresis mass spectrometry to the characterization of bacterial lipopolysaccharidesMASS SPECTROMETRY REVIEWS, Issue 1 2007Jianjun Li Abstract Capillary electrophoresis (CE) is a high-resolution technique for the separation of complex biological mixtures and has been widely applied to biological analyses. The coupling of capillary electrophoresis with mass spectrometry (MS) provides a powerful approach for rapid identification of target analytes present at trace levels in biological matrices, and for structural characterization of complex biomolecules. Here we review the analytical potential of combined capillary electrophoresis electrospray mass spectrometry (CE-MS) for the analysis of bacterial lipopolysaccharides (LPS). This hyphened methodology facilitates the determination of closely related LPS glycoform and isoform families by exploiting differences in their unique molecular conformations and ionic charge distributions by electrophoretic separation. On-line CE-MS also provides an additional avenue to improve detection limits, which has been successfully applied to directly probe oligosaccharide LPS glycoform populations of bacteria isolated from infected animal models without the need for further passage. © 2006 Wiley Periodicals, Inc., Mass Spec Rev 26:35,50, 2007 [source] Variation in 16S-23S rRNA intergenic spacer regions among Bacillus subtilis 168 isolatesMOLECULAR MICROBIOLOGY, Issue 1 2001Yevette J. Shaver The genome of the Bacillus subtilis 168-type strain contains 10 ribosomal RNA (rRNA) operons. In the intergenic spacer region (ISR) between the 16S and 23S rRNA genes, five rRNA operons, rrnI-H-G and rrnJ-W, lack a trinucleotide signature region. Precise determination of molecular weight (MW), using electrospray mass spectrometry (MS), of the polymerase chain reaction (PCR) products from a segment of the ISR from the 168-type strain and B. subtilis 168-like strain 23071 demonstrated 114 and 111 basepair (bp) PCR products (due to the presence or absence of the insert in the operons) as predicted from sequence. However, PCR of the ISR segment for five other B. subtilis 168 isolates generated only a 114 bp PCR product, suggesting the presence of the trinucleotide signature region in all rRNA operons for these strains. Additional genetic variability between the seven B. subtilis 168 isolates was demonstrated by restriction fragment length polymorphism (RFLP) of the rRNA operons, with three distinct patterns found upon Southern blot analysis. The 168-type strain and three others (23066, 23067, and 23071) exhibited the same Southern pattern. Thus, operon deletion is not responsible for the absence of a 111 bp product on MS analysis for strains 23066 and 23067. Restriction analysis confirmed the presence of the trinucleotide signature region in the ISR of all rRNA operons for five B. subtilis 168 isolates; sequencing of rrnW/H from a representative strain also upheld this finding. These results help provide a better understanding of variations in sequence, operon number and chromosomal organization, both within a genome and among isolates of B. subtilis subgroup 168. It is also hypothesized that the presence of the trinucleotide insert in certain rRNA operons may play a role in rRNA maturation and protein synthesis. [source] Characterisation of fungal lanostane-type triterpene acids by electrospray ionisation mass spectrometryPHYTOCHEMICAL ANALYSIS, Issue 6 2007Gabriela M. Cabrera Abstract Lanostane-triterpene acids obtained from the culture of the fungus Coriolellus malicola were studied by electrospray mass spectrometry in the negative ion mode using quadrupole time-of-flight and quadrupole ion trap analysers. Despite the differences observed in the mass spectra recorded with these instruments, a set of fragment ions was found to be characteristic of the family, depending on the ,7,9(11) or ,8 skeleton and the particular functional group at C-3. Copyright © 2007 John Wiley & Sons, Ltd. [source] Detection of four oxidation sites in viral prolyl-4-hydroxylase by top-down mass spectrometryPROTEIN SCIENCE, Issue 10 2003Ying Ge Abstract Oxidative inactivation is a common problem for enzymatic reactions that proceed via iron oxo intermediates. In an investigation of the inactivation of a viral prolyl-4-hydroxylase (26 kD), electrospray mass spectrometry (MS) directly shows the degree of oxidation under varying experimental conditions, but indicates the addition at most of three oxygen atoms per molecule. Thus, molecular ion masses (M + nO) of one sample indicate the oxygen atom adducts n = 0, 1, 2, 3, and 4 of 35, 41, 19, 5 ± 3, and <2%, respectively; "top-down" MS/MS of these ions show oxidation at the sites R28,V31, E95,F107, and K216 of 22%, 28%, and 34%, respectively, but with a possible (,4%) fourth site at V125,D150. However, for the doubly oxidized molecular ions (increasing the precursor oxygen content from 0.94 to 2), MS/MS showed an easily observable ,13% oxygen at the V125,D150 site. For the "bottom-up" approach, detection of the ,4% oxidation at the V125,D150 site by MS analysis of a proteolysis mixture would have been very difficult. The unmodified peptide containing this site would represent a few percent of the proteolysis mixture; the oxidized peptide not only would be just ,4% of this, but the uniqueness of its mass value (,1,2 kD) would be far less than the 11,933 Dalton value used here. Using different molecular ion precursors for top-down MS/MS also provides kinetic data from a single sample, that is, from molecular ions with 0.94 and 2 oxygens. Little oxidation occurs at V125,D150 until K216 is oxidized, suggesting that these are competitively catalyzed by the iron center; among several prolyl-4-hydroxylases the K216, H137, and D139 are conserved residues. [source] Using nondenaturing mass spectrometry to detect fortuitous ligands in orphan nuclear receptorsPROTEIN SCIENCE, Issue 4 2003Noelle Potier Abstract Nondenaturing electrospray mass spectrometry (ESI-MS) has been used to reveal the presence of potential ligands in the ligand-binding domain (LBD) of orphan nuclear receptors. This new approach, based on supramolecular mass spectrometry, allowed the detection and identification of fortuitous ligands for the retinoic acid-related orphan receptor , (ROR,) and the ultraspiracle protein (USP). These fortuitous ligands were specifically captured from the host cell with the proper stoichiometry. After organic extraction, these molecules have been characterized by classic analytical methods and identified as stearic acid for ROR, and a phosphatidylethanolamine (PE) for USP, as confirmed by crystallography. These molecules act as "fillers" and may not be the physiological ligands, but they prove to be essential to stabilize the active conformation of the LBD, enabling its crystallization. The resulting crystal structures provide a detailed picture of the ligand-binding pocket, allowing the design of highly specific synthetic ligands that can be used to characterize the function of orphan nuclear receptors. An additional advantage of this new method is that it is not based on a functional test and that it can detect low-affinity ligands. [source] Negative ion fragmentations of deprotonated peptides.RAPID COMMUNICATIONS IN MASS SPECTROMETRY, Issue 13 2009The unusual case of isoAsp: a joint experimental, theoretical study. The following peptides have been examined in this study: GLDFG(OH), caeridin 1.1 [GLLDGLLGLGGL(NH2)], 11 Ala citropin 1.1 [GLFDVIKKVAAVIGGL(NH2)], Crinia angiotensin [APGDRIYVHPF(OH)] and their isoAsp isomers. It is not possible to differentiate between Asp- and isoAsp-containing peptides (used in this study) using negative ion electrospray mass spectrometry. This is because the isoAsp residue cleaves to give the same fragment anions as those formed by , and , backbone cleavage of Asp. The isoAsp fragmentations are as follows: RNHCH(CO2H),CHCONHR,,,,[RNH,(HO2CCHCHCONHR,)],,,RNH,+HO2CCHCHCONHR, and RNHCH(CO2H),CHCONHR,,,,[RNH,(HO2CCHCHCONHR,],,,,O2CCHCHCONHR,+RNH2. Calculations at the HF/6-31+G(d)//AM1 level of theory indicate that the first of these isoAsp cleavage processes is endothermic (by +115,kJ mol,1), while the second is exothermic (,85,kJ mol,1). The barrier to the highest transition state is 42,kJ mol,1. No diagnostic cleavage cations were observed in the electrospray mass spectra of the MH+ ion of the Asp- and isoAsp-containing peptides (used in this study) to allow differentiation between these two amino acid residues. Copyright © 2009 John Wiley & Sons, Ltd. [source] | |||||||||||||||||||||||||||||||||||||