Observation and implications of high mass-to-charge ratio ions from electrospray ionization mass spectrometry

High mass-to-charge ratio ions (> 4000) from electrospray ionization (ESI) have been observed for several proteins, including bovine cytochrome c (M _r 12,231) and porcine pepsin (M _r 34,584), by using a quadrupole mass spectrometer with an m/z 45,000 range. The ESI mass spectrum for cytochrome c in an aqueous solution gives a charge state distribution that ranges from 12 + to 2 +, with a broad, low-intensity peak in the mass-to-charge ratio region corresponding to the [M + H]⁺ ion. the negative ion ESI mass spectrum for pepsin in 1% acetic acid solution shows a charge state distribution ranging from 7? to 2?. To observe the [M - H]^? ion, harsher desolvation and interface conditions were required. Also observed was the abundant aggregation of the protens with average charge states substantially lower than observed for their monomeric counterparts. The negative ion ESI mass spectrum for cytochrome c in 1–100 mM NH₄OAc solutions showed greater relative abundances for the higher mass-to-charge ratio ions than in acuidic solutions, with an [M - H]^? ion relative abundance approximately 50% that of the most abundant charge state peak. The observation that protein aggregates are formed with charge states comparable to monomeric species (at fower mass-to-charge ratios) suggests that the high mass-to-charge ratio monomers may be formed by the dissociation of aggregate species. The observation of low charge state and aggregate molecular ions concurrently with highly charged species may serve to support a variation of the charged residue model, originally described by Dole and co-workers (Dole, M., et al. J. Chem. Phys. 1968, 49, 2240; Mack, L. L., et al. J. Chem. Phys. 1970, 52, 4977) which involves the Coulombically driven formation of either very highly solvated molecular ions or lower ananometer-diameter droplets.     

Liquid chromatography/thermospray mass spectrometry of monosaccharides and their derivatives

Thermospray (TSP) mass spectrometry has proved to be a useful technique for analysing various highly polar compounds. The use of a quadrupole mass spectrometer equipped with a thermospray/plasmaspray interface in the analysis of more than 30 monosaccharides and sugar derivatives is described. A 1:1 mixture of methanol or acetonitrile and 0.1 M aqueous ammonium acetate as eluent at 1 cm³ min^?1 affords the best results. The correct setting of the capillary tip temperature and repeller voltage was fundamental for the ionization of carbohydrates. The/optimum values of these parameters were 240–250°C and 220–240 V, respectively. The thermospray mass spectra of most carbohydrates exhibit strong [M + NH₄]⁺ ions which provide molecular mass information. The underivatized and derivatized monosaccharides could be grouped according to the presence or absence and the relative abundances of [M + NH₄ ? H₂O]⁺, [M + H]⁺ and [M + NH₄]⁺ ions.     

Effect of ammonium formate as ionizing additive in thermospray liquid chromatography-mass spectrometry for the determination of triazine,phenylurea and chlorinated phenoxyacetic acid herbicides

A comparison between the use of ammonium acetate and ammonium formate in thermospray liquid chromatography-mass spectrometry with positive and negative ion modes using ‘filament-on’ mode has been applied for the determination of simazine, atrazine, propazine, monuron, diuron, linuron, 2,4,-D, 2,4,5-T and silvex. By using ammonium formate, the positive ion mode showed for triazine and phenylurea herbicides [M + H]⁺ and [M + NH₄]⁺, respectively, and the formation of other adduct ions different from ammonium acetate. In the negative ion mode, chlorinated phenoxyacetic acid herbicides exhibited [M + acetate]^? or [M + formate]^?, depending on the ionizing additive. Applications are reported for the determination of triazine and chlorinated phenoxyacetic acid herbicides in spiked soil and water samples, respectively.     

Unique thermospray mass spectrometry of 1,4-benzoquinone and analogs in ammonium acetate solutions

In general, ions corresponding to [M + H]⁺ and/or [M + NH₄]⁺ are observed in thermospray mass spectrometry (TSMS) when using ammonium acetate in the liquid carrier. For several quinones investigated, unique thermospray mass spectra were detected with a mass spectral peak corresponding to an [M + 16]⁺ ion being observed in aqueous ammonium acetate solutions. Investigation of l,4-benzoquinone (BQU) and structurally analogous quinones indicated that amine conjugate formation with BQU and similar quinones was the origin of the unique [M + 16]⁺ ion in TSMS. When methanol was added to the liquid carrier, ions corresponding to methoxy conjugation were detected. High-performance liquid chromatography followed by TSMS or electrochemical detection gave evidence that this amine and methoxy conjugate formation was occurring in the thermospray source area.     

Oxidation reactions in triterpenes under chemical ionization conditions

From a collisional activation spectral study it has been found that certain triterpene alcohols with an ursane or oleanane skeleton undergo oxidation to the corresponding ketones under chemical ionization (NH₃) conditions giving rise to abundant [M + NH₄ ? 2]⁺ ions. Mass-analysed ion kinetic energy and B²/E scan results indicate that both [M + NH₄]⁺ and [M + N₂H₇ ? 2]⁺ ions contribute to the formation of the [M + NH₄ ? 2]⁺ ion.     

Native Electrospray Mass Spectrometry of DNA G-Quadruplexes in Potassium Solution

A commonly used electrolyte in electrospray mass spectrometry (ESI-MS) of biomolecules is ammonium acetate (NH₄OAc). Although some nucleic acid structures such as duplexes require only proper physiological ionic strength (whatever the monovalent ions) to be properly folded in ESI-MS conditions, the folding of some other nucleic acid structures such as DNA G-quadruplexes also depends on direct binding of specific cations. Here, we developed ESI-MS compatible conditions that allow one to observe DNA G-quaduplexes with K⁺ ions specifically bound between G-quartets. NH₄OAc was replaced with trimethylammonium acetate (TMAA), at concentrations up to 150 mM to provide physiological ionic strength, and the solution was doped with KCl at concentrations up to 1 mM. The trimethylammonium ion is too large to coordinate between G-quartets, where only K⁺ ions bind. Compared with the equivalent NH₄OAc/KCl mixtures, the TMAA/KCl mixtures provide cleaner spectra by suppressing the nonspecific adducts, and favor the formation of similar stacking arrangements as in 100 mM KCl (physiologically relevant cation) for the polymorphic human telomeric DNA G-quadruplexes. This new sample preparation method can be exploited to determine the number of potassium binding sites in new sequences, to screen ligand binding to the structures favored in potassium, and to transfer potassium-bound G-quadruplexes to the mass spectrometer for gas-phase structural probing, as illustrated herein with ion mobility spectrometry experiments.

Ion–molecule reaction in the gas phase 3—nucleophilic substitution of 17ξ-R-5α,14β-androstane-14,17ξ-diols under [NH4]+ chemical ionization conditions1

Under Ammonia chemical Ionization conditions the source decompositions of [M + NH₄]⁺ ions formed from epimeric tertiary steroid alchols 14 OH_β, 17OH_α or 17 OH_β substituted at position 17 have been studied. They give rise to formation of [M + NH₄? H₂O]⁺ dentoed as [MH_sH]⁺, [M_sH? H₂O]⁺, [M_sH? NH₃]⁺ and [M_sH? NH₃? H₂O]⁺ ions. Stereochemical effects are observed in the ratios [M_sH? H₂O]⁺/[M_sH? NH₃]⁺. These effects are significant among metastable ions. In particular, only the [M_sH]⁺ ions produced from trans-diol isomers lose a water molecule. The favoured loss of water can be accounted for by an S_N2 mechanism in which the insertion of NH₃ gives [M_sH]⁺ with Walden inversion occurring during the ion-molecule reaction between [M + NH₄]⁺ + NH₃. The S_N1 and S_Ni pathways have been rejected.     

Mass spectra of sulfinamide derivatives and identification of their thermal decomposition products

The mass spectra of 30 sulfinamide derivatives (RSONHR', R' alkyl or p-XC₆H₄) are reported. Most of the spectra had peaks attributable to thermal decomposition products. For some compounds these were identified by pyrolysis under similar conditions to be: RSO₂NHR', RSO₂SR, RSSR and NH₂R' (in all kinds of sulfinyl amides); RSNHR' (in the case of arylsulfinyl arylamides); RSO₂C₆H₄NH₂, RSOC₆H₄NH₂ and RSC₆H₄NH₂ (in the case of arylsulfinyl arylamides of the type of X = H) The mass spectra of the three thermally stable compounds showed that there are several kinds of common fragment ions. The mass spectra of the thermally labile compounds had two groups of ions; (i) characteristic fragment ions of the intact molecules and (ii) the molecular ions of the thermal decomposition products. It was concluded that the sulfinamides give the following ions after electron impact: [M]⁺, [M ? R]⁺, [M ? R + H]⁺, [M ? SO]⁺, [RS]⁺, [NHR']⁺, [NHR' + H]⁺, [RSO]⁺, [RSO + H]⁺, [R]⁺, [R + H]⁺, [R']⁺ and [M ? OH]⁺, and that the thermal decomposition products give the following ions: [RSO₂SR]⁺, [RSSR]⁺, [M ? O]⁺, [M + O]⁺ and [RSOC₆H₄NH₂]⁺.     

Synthesis of dirhodium[3H]tetraacetate

Realizing a need for labeled dirhodium tetraacetate [Rh₂/OAc/₄] for binding studies by the equilibrium dialysis procedure, we have established a method for the preparation and purification of [³H]Rh₂/OAc/₄. This is obtained with a tritium label of a sufficiently high specific activity in the methyl group of acetate residues. The method consists of replacement of the existing acetate bridge by [³H]OAc^–. A typical preparation involves refluxing Rh₂/OAc/₄ with [³H]NaOAc in dry ethanol at 80°C for 6 h. The reaction time is critical for obtaining the product with a high specific activity. A simple purification of reaction products yields the compound of interest with a high specific activity, i. e., 315±10 Ci per mol of Rh₂/OAc/₄ and in satisfactory yield /87% of the starting material., This labeled material can be synthesized with greatly increased specific activity /of tritium in acetate groups/ by employing [³H]NaOAc without prior dilution. The labeled Rh₂/OAc/₄ is stable and yields a characteristic product with adenylic acid.     

Synthese und Struktur der ternären Ammoniumnitrate (NH4)2[M(NO3)5] (M = Tb?Lu,Y

Synthesis and Structure of the Ternary Ammonium Nitrates (NH₄)₂[M(NO₃)₅] (M = Tb? Lu, Y) Single crystals of the ternary ammonium nitrates (NH₄)₂[M(NO₃)₅] (M = Tb? Lu, Y) are obtained from the solution of the sesquioxides in a melt of NH₄NO₃ and sublimation of the excess NH₄NO₃. In the crystal structure of (NH₄)₂[Tm(NO₃)₅] (trigonal, P3₁, Z = 3; a = 1 123.76(8), c = 930.1(1) pm; R = 0.062; R_w = 0.034) Tm³⁺ is surrounded by five bidentate nitrate ligands. The isolated [Tm(NO₃)₅]^2? groups are held together by ammonium ions.     

Detection and identification of hydrophilic selenium compounds in selenium-rich yeast by size exclusion-microbore normal-phase HPLC with the on-line ICP-MS and electrospray Q-TOF-MS detection

Normal-phase HPLC and hydrophilic interaction HPLC (HILIC) were investigated for the separation of selenometabolites in a water extract of Se-rich yeast prior to their detection by ICP-MS and identification by electrospray MS/MS. The targeted fraction was a low-abundant fraction co-eluting with salt and sulfur analogues in size-exclusion chromatography which has so far been inaccessible to Se speciation studies. The optimization of the separation conditions resulted in the highest separation efficiency when HILIC was used and elution was carried out isocratically with a low concentration ammonium acetate buffer (1 mM ammonium acetate/10 mM acetic acid) in 80% acetonitrile. Out of 15 peaks observed with the Se-specific ICP-MS detection 12 was identified by electrospray Q-TOF MS/MS (2,3-dihydroxypropionyl (DHP)-Se-methylselenocysteine [M+H]⁺: 272, Se-methyl-γ-glutamyl-selenocysteinylglycine dioxide [M+H]⁺: 402, γ-glutamyl-Se-methylselenocysteine [M+H]⁺: 313; isomers of γ-glutamylselenocystathionine [M+H]⁺: 400; Se-methyl-selenoglutathione [M+H]⁺: 370, isomers of N-acetylselenocystathionine [M+H]⁺: 313, 2,3-DHP-selenohomolanthionine [M+H]⁺: 373, isomers of 2,3-DHP-selenocystathionine [M+H]⁺: 359, 2,3-DHP-selenolanthionine [M+H]⁺: 345 and selenohomolanthionine [M+H]⁺: 285).     

Chemical ionization and collisional activation spectra of α,β-unsaturated nitriles

A study of the chemical ionization (CI) and collisional activation (CA) spectra of a number of α, β-unsaturated nitriles has revealed that the even-electron ions such as [MH]⁺ and [MNH₄]⁺ produced under chemical ionization undergo decomposition by radical losses also. This results in the formation of M ⁺˙ ions from both [MH]⁺ and [MNH₄]⁺ ions. In the halogenated molecules losses of X˙ and HX compete with losses of H˙ and HCN. Elimination of X˙ from [MH]⁺ is highly favoured in the bromoderivative. The dinitriles undergo a substitution reaction in which one of the CN groups is replaced with a hydrogen radical and the resulting mononitrile is ionized leading to [M ? CN + 2H]⁺ under CI(CH₄) or [M ? CN + H + NH₄] and [M ? CN + H + N₂H₇]⁺ under CI(NH₃) conditions.     

Factors affecting reactivity in ammonia chemical ionization mass spectrometry

Several factors affecting reactivity in ammonia chemical ionization mass spectrometry (NH₃ CI) have been examined. These include the sample proton affinity, the preferred site of protonation and [NH₄]⁺ attachment, and substituent effects. In general, compounds having proton affinities ?787 kJ mol^?1 do not yield analytically useful intensities of the [M·NH₄]⁺ adduct ion. Substituted aromatic compounds in which the ring is the most basic site yield little (if any) [M·NH₄]⁺ ion even if the proton affinity of the compound is greater than 787 kJ mol^?1. On the other hand, some aromatic compounds in which the substituent is the most basic site yield relatively abundant adduct ions. The spectra of compounds possessing a good leaving group (X) exhibit only weak [M·NH₄]⁺ ions, but intense [M·NH₄ ? HX]⁺ and [M ? X]⁺ ions formed by substitution and elimination reactions. Electronic effects strongly influence these processes. Several examples are presented in which isomers are readily differentiated because of different reactivities under ammonia chemical ionization conditions.     

Ammonia in the ion source. II. Clustering with aromatic nitro compounds

Under positive ion chemical ionization conditions with ammonla at relatively low pressure, aromatic nitro compounds do not form [M + H]⁺ ions but often form ionic clusters [M + NH₄]⁺ and [M + N₂H₇]⁺. Nitrobenzene forms a cluster [2M + NH₄]⁺ and aniline, formed by nucleophilic substitution, leads to a cluster [anilinium ion + nitrobenzene]⁺. The dinitrobenzenes form [M + NH₄]⁺ clusters and show evidence of nitroaniline formation and clustering. 1,3,5-Trinitrobenzene gives little indication of clustering or of substitution. The six isomers of trinitrotoluene appear to be stabilized by the methyl group and form clusters up to [M + N₃H₁₀]⁺. Nucleophilic substitution leads to dinitrotoluidines, which also form clusters with ammonium ions.     

Influence of reversed- and normal-phase liquid chromatographic eluents in the fragmentation of selected chlorinated herbicides in thermospray liquid chromatography-mass spectrometry

The effect of two completely different mobile phase compositions, reversed-phase acetonitrile-water + ammonium acetate and normal-phase cyclohexane, were compared in filament-on thermospray liquid chromatography-mass spectrometry (LC-MS) for the determination of selected chlorinated herbicides such as chloroatrazines and chlorinated phenoxyacetic acids. By using acetonitrile-water + 0.05 M ammonium acetate mixtures in positive ion mode thermospray LC-MS, the chloroatrazine herbicides showed the acetonitrile adduct ion [M + (CH₃CN)H]⁺ as the base peak, whereas the chlorinated phenoxyacetic acids showed no signal. In contrast, when cyclohexane, which is reported for the first time as an eluent in the thermospray technique, was used as the mobile phase the chlorinated phenoxyacetic acid herbicides exhibited [M – H]⁺, [M – Cl]⁺ and M⁺˙ as the main ions. Negative ion mode thermospray LC-MS showed [M – H]^? as the base peak for the chloroatrazines in the different mobile phases, whereas the chlorinated phenoxyacetic acids exhibited [M + H]^?, [M + Cl]^? or [M – HCl]^? as the base peaks in cyclohexane and [M + acetate]^? in acetonitrile-water-ammonium acetate.     

Solvation and Ion-Pairing Effects of Choline Acetate Electrolyte in Protic and Aprotic Solvents Studied by NMR Titrations

Choline-based electrolytes have been proposed as environmentally friendly and low-cost alternatives for secondary zinc air batteries. Choline acetate [Ch]⁺[OAc]⁻ in protic (D₂O) and aprotic (DMSO-d₆) solvents has been studied by means of concentration-dependent ¹H NMR, viscosity, and density measurements. The viscosities have been calculated on the basis of the Jones-Dole equation and showed that the dominant contribution originates from short-range ion-solvent interactions. Site-specific association affinities were assigned from NMR chemical shift titrations. In DMSO-d₆, the hydroxyl group of choline was found to have the smallest dissociation constant followed by the methyl group of acetate. The corresponding Gibbs energies at low concentration were found to be in agreement with a solvent-separated ion pair (2SIP) configuration, whereas at concentrations above 300 mM, a solvent-shared ion pair (SIP) configuration was assigned. For [Ch]⁺[OAc]⁻ in D₂O, association effects were found to be weaker, attributed to the high dielectric constant of the solvent. On time scales on the order of 100 ms, NMR linewidth perturbations indicated a change in the local rotational dynamics of the ions, attributed to short-range cation-solvent interactions and not to solvent viscosity. At 184 mM, 40 % of the cations in DMSO-d₆ and 10 % in D₂O were found to exhibit short-range interactions, as indicated by the linewidth perturbations. It was found that at about 300 mM, the ions in DMSO-d₆ exhibit a transition from free to collective translational dynamics on time scales on the order of 400 ms. In DMSO-d₆, both ions were found to be almost equally solvated, whereas in D₂O solvation of acetate was stronger, as indicated by the obtained effective hydrodynamic radii. For [Ch]⁺[OAc]⁻ in DMSO-d₆, the results suggest a solvent-shared ion association with weak H-bonding interactions for concentrations between 0.3–1 M. Overall, the extent of ion association in solvents such as DMSO is not expected to significantly limit charge transport and hinder the performance of choline-based electrolytes.     

Ionization and collision induced dissociation of steroid bisglucuronides

Studies on steroid metabolism are of utmost importance to improve the detection capabilities of anabolic androgenic steroids (AASs) misuse in sports drug testing. In humans, glucuronoconjugates are the most abundant phase II metabolites of AAS. Bisglucuronidation is a reaction where two separated functional groups on the same molecule are conjugated with glucuronic acid. These metabolites have not been studied in depth for steroids and could be interesting markers for doping control. The aim of the present work was to study the ionization and collision‐induced dissociation of steroid bisglucuronides to be able to develop mass spectrometric analytical strategies for their detection in urine samples after AAS administration. Because steroid bisglucuronides are not commercially available, 19 of them were qualitatively synthesized to study their mass spectrometric behavior. Bisglucuronides ionized as [M+NH₄]⁺ in positive mode, and as [M–H]⁻ and [M–2H]²⁻ in negative mode. The most specific product ions of steroid bisglucuronides in positive mode resulted from the neutral losses of 387 and 405 Da (corresponding to [M+NH₄–NH₃–2gluc–H₂O]⁺ and [M+NH₄–NH₃–2gluc–2H₂O]⁺, respectively, being “gluc” a dehydrated glucuronide moiety), and in negative mode, the fragmentation of [M–2H]²⁻ showed ion losses of m /z 175 and 75 (gluc⁻ and HOCH₂CO₂⁻, respectively). On the basis of the common behavior, a selected reaction monitoring method was developed to detect bisglucuronide metabolites in urine samples. As a proof of concept, urines obtained after administration of norandrostenediol were studied, and a bisglucuronide metabolite was detected in those urines. The results demonstrate the usefulness of the analytical strategy to detect bisglucuronide metabolites in urine samples, and the formation of these metabolites after administration of AAS.     

Characterization of C8H10 alkylbenzenes by negative ion mass spectrometry

The O^?˙ chemical ionization mass spectrri of the C₈H₁₀ alkylbenzenes, o-, m-. andp -xylene and ethylbenzene, show formation of [M ? H + O]^?, [M ? H]^?, [M ? H₂]^?˙ and, for the xylenes, [M ? CH₃ + O]^? as primary reaction products; the relative importance of these products depends on the isomer. However, [OH]^? is a primary product from reaction of O^?˙ with both the C₈H₁₀ isomers and hydrogen-containing impurities; [OH]^? reacts further with the alkylbenzenes to produce [M ? H]^? with the result that the chemical ionization mass spectra depend on experimental conditions such as sample size and the presence of impurities. The collision-induced charge inversion mass spectra of the [M ? H + O]^? and [M ? H]^? products allow only distinction of ethylbenzene from the xylenes. However, the collision-induced charge inversion mass spectra of the [M ? H₂]^?˙ ions show differences which allow identification of each isomer.     

Ammonium adduct ion in ammonia chemical ionization mass spectrometry: 2—Mechanism of elimination of neutrals from the ammonium adduct ion

The mechanism of elimination of ROH (R = H or CH₃) from the ammonium adduct ion, [M+NH₄]⁺, of 1-adamantanol and its methyl ether is examined by using linked-scan metastable ion spectra and by measuring the dependence of the peak intensity ratio [M+NH₄]⁺/[M+NH₄? ROH]⁺ on ammonia pressure. For 1-adamantanol both S_Ni and S_N1 reactions are suggested in metastable ion decomposition, while only the S_N1 mechanism is operative in the ion source. For 1-adamantanol methyl ether the S_N1 reaction predominates both in metastable ion decomposition and in the ion source reaction.     

Ion formation of N-Methyl carbamate pesticides in thermospray mass spectrometry: The effects of additives to the liquid chromatographic eluent and of the vaporizer temperature

The effects of three additives—ammonium acetate, ammonium formate, and nicotinic acid—to the liquid chromatographic (LC) eluent and of the vaporizer temperature on the ion formation of N-methyl carbamate pesticides in thermospray (TSP) mass spectrometry was investigated by using filament- or discharge-assisted ionization. Nineteen carbamates and 12 of their known environmental degradation products were used as model compounds. The additives cause a strong reduction in the abundance of the characteristic fragment ions [M + H ? CH₃NCO]⁺ and [M ? H ? CH₃NCO]^? for some of the carbamates. The addition of nicotinic acid reduces the quasimolecular ion intensity and, in most cases, produces nicotinic acid adduct ions. The addition of ammonium acetate or ammonium formate increases the intensity of the quasimolecular ion and in most cases produces a base peak for the ammonium adduct ion. The combination of a suppression of fragmentation and an enhancement of quasimolecular ion formation produces an overall gain in sensitivity. As to more specific effects, the addition of the ammonium salts reduces the intensity of M^?? with the chlorinated carbamate barban and suppresses the formation of “odd” adduct ions in the TSP mass spectra of most other carbamates. Monitoring the intensity of the fragment and the quasimolecular ion signal as a function of the probe stem temperature, and the related probe tip temperature, proved to be an easy method to study the thermal degradation of the carbamates. This monitoring procedure showed that methiocarb and its sulfone already suffer from thermal degradation at a stem temperature of 90°C and that these compounds will therefore present problems in quantitation with LC/TSP mass spectrometry.