Without any sample pretreatment, effervescent beverage fluids were manually sprayed into the primary ion plume created by
using a nanoelectrospray ionization source for direct ionization, and the analyte ions of interest were guided into an ion
trap mass spectrometer for tandem mass analysis. Functional ingredients (e.g., vitamins, taurine, and caffeine, etc.) and
spiked impurity (e.g., cocaine) in various beverages, such as Red Bull energy drink, Coco-cola, and Pepsi samples were rapidly
identified within 1.5 s. The limit of detection was found to be 7 ∼ 15 fg (S/N = 3) for cocaine in different samples using the characteristic fragment (m/z 150) observed in the MS3 experiments. Typical relative standard deviation and recovery of this method were 6.9% ∼ 8.6% and 104% ∼ 108% for direct
analysis of three actual samples, showing that nanoextractive electrospray ionization tandem mass spectrometry is a useful
technique for fast screening cocaine presence in beverages. 相似文献
Tandem mass spectral library searching is finding increased use as an effective means of determining chemical identity in mass spectrometry-based omics studies. We previously reported on constructing a tandem mass spectral library that includes spectra for multiple precursor ions for each analyte. Here we report our method for expanding this library to include MS2 spectra of fragment ions generated during the ionization process (in-source fragment ions) as well as MS3 and MS4 spectra. These can assist the chemical identification process. A simple density-based clustering algorithm was used to cluster all significant precursor ions from MS1 scans for an analyte acquired during an infusion experiment. The MS2 spectra associated with these precursor ions were grouped into the same precursor clusters. Subsequently, a new top-down hierarchical divisive clustering algorithm was developed for clustering the spectra from fragmentation of ions in each precursor cluster, including the MS2 spectra of the original precursors and of the in-source fragments as well as the MSn spectra. This algorithm starts with all the spectra of one precursor in one cluster and then separates them into sub-clusters of similar spectra based on the fragment patterns. Herein, we describe the algorithms and spectral evaluation methods for extending the library. The new library features were demonstrated by searching the high resolution spectra of E. coli extracts against the extended library, allowing identification of compounds and their in-source fragment ions in a manner that was not possible before.
We report here an automated method for the identification of N-oxide functional groups in drug metabolites by using the combination
of liquid chromatography/tandem mass spectrometry (LC/MSn) based on ion-molecule reactions and collision-activated dissociation (CAD). Data-dependent acquisition, which has been readily
utilized for metabolite characterization using CAD-based methods, is adapted for use with ion-molecule reaction-based tandem
mass spectrometry by careful choice of select experimental parameters. Two different experiments utilizing ion-molecule reactions
are demonstrated, data-dependent neutral gain MS3 and data-dependent neutral gain pseudo-MS3, both of which generate functional group selective mass spectral data in a single experiment and facilitate increased throughput
in structural elucidation of unknown mixture components. Initial results have been generated by using an LC/MSn method based on ion-molecule reactions developed earlier for the identification of the N-oxide functional group in pharmaceutical
samples, a notoriously difficult functional group to identify via CAD alone. Since commercial software and straightforward,
external instrument modification are used, these experiments are readily adaptable to the industrial pharmaceutical laboratory. 相似文献
Improved methods for structural analyses of glycosaminoglycans (GAGs) are required to understand their functional roles in
various biological processes. Major challenges in structural characterization of complex GAG oligosaccharides using liquid
chromatography-mass spectrometry (LC-MS) include the accurate determination of the patterns of sulfation due to gas-phase
losses of the sulfate groups upon collisional activation and inefficient on-line separation of positional sulfation isomers
prior to MS/MS analyses. Here, a sequential chemical derivatization procedure including permethylation, desulfation, and acetylation
was demonstrated to enable both on-line LC separation of isomeric mixtures of chondroitin sulfate (CS) oligosaccharides and
accurate determination of sites of sulfation by MSn. The derivatized oligosaccharides have sulfate groups replaced with acetyl groups, which are sufficiently stable to survive
MSn fragmentation and reflect the original sulfation patterns. A standard reversed-phase LC-MS system with a capillary C18 column
was used for separation, and MSn experiments using collision-induced dissociation (CID) were performed. Our results indicate that the combination of this
derivatization strategy and MSn methodology enables accurate identification of the sulfation isomers of CS hexasaccharides with either saturated or unsaturated
nonreducing ends. Moreover, derivatized CS hexasaccharide isomer mixtures become separable by LC-MS method due to different
positions of acetyl modifications. 相似文献
In contrast to GC-MS libraries, currently available LC-MS libraries for toxicological detection contain besides parent drugs
only some main metabolites limiting their applicability for urine screening. Therefore, a metabolite-based LC-MSn screening procedure was developed and exemplified for antidepressants. The library was built up with MS2 and MS3 wideband spectra using an LXQ linear ion trap with electrospray ionization in the positive mode and full-scan information-dependent
acquisition. Pure substance spectra were recorded in methanolic solution and metabolite spectra in urine from rats after administration
of the corresponding drugs. After identification, the metabolite spectra were added to the library. Various drugs and metabolites
could be sufficiently separated. Recovery, process efficiency, matrix effects, and limits of detection for selected drugs
were determined using protein precipitation. Automatic data evaluation was performed using ToxID and SmileMS software. The
library consists of over 700 parent compounds including 45 antidepressants, over 1,600 metabolites, and artifacts. Protein
precipitation led to sufficient results for sample preparation. ToxID and SmileMS were both suitable for target screening
with some pros and cons. In our study, only SmileMS was suitable for untargeted screening being not limited to precursor selection.
The LC-MSn method was suitable for urine screening as exemplified for antidepressants. It also allowed detecting unknown compounds based
on known fragment structures. As ion suppression can never be excluded, it is advantageous to have several targets per drug.
Furthermore, the detection of metabolites confirms the body passage. The presented LC-MSn method complements established GC-MS or LC-MS procedures in the authors’ lab. 相似文献
Cationic metal ion-coordinated N-diisopropyloxyphosphoryl dipeptides (DIPP-dipeptides) were analyzed by electrospray ionization multistage tandem mass spectrometry
(ESI-MSn). Two novel rearrangement reactions with hydroxyl oxygen or carbonyl oxygen migrations were observed in ESI-MS/MS of the
metallic adducts of DIPP-dipeptides, but not for the corresponding protonated DIPP-dipeptides. The possible oxygen migration
mechanisms were elucidated through a combination of MS/MS experiments, isotope (18O, 15N, and 2H) labeling, accurate mass measurements, and density functional theory (DFT) calculations at the B3LYP/6-31 G(d) level. It
was found that lithium and sodium cations catalyze the carbonyl oxygen migration more efficiently than does potassium and
participation through a cyclic phosphoryl intermediate. In addition, dipeptides having a C-terminal hydroxyl or aromatic amino
acid residue show a more favorable rearrangement through carbonyl oxygen migration, which may be due to metal cation stabilization
by the donation of lone pair of the hydroxyl oxygen or aromatic π-electrons of the C-terminal amino acid residue, respectively.
It was further shown that the metal ions, namely lithium, sodium, and potassium cations, could play a novel directing role
for the migration of hydroxyl or carbonyl oxygen in the gas phase. This discovery suggests that interactions between phosphorylated
biomolecules and proteins might involve the assistance of metal ions to coordinate the phosphoryl oxygen and protein side
chains to achieve molecular recognition. 相似文献
It has previously been reported that disulfide and backbone bonds of native intact proteins can be concurrently cleaved using
electrospray ionization (ESI) and collision-induced dissociation (CID) tandem mass spectrometry (MS/MS). However, the cleavages
of disulfide bonds result in different cysteine modifications in product ions, making it difficult to identify the disulfide-bonded
proteins via database search. To solve this identification problem, we have developed a pseudo MS3 approach by combining nozzle-skimmer dissociation (NSD) and CID on a quadrupole time-of-flight (Q-TOF) mass spectrometer
using chicken lysozyme as a model. Although many of the product ions were similar to those typically seen in MS/MS spectra
of enzymatically derived peptides, additional uncommon product ions were detected including ci-1 ions (the ith residue being aspartic acid, arginine, lysine and dehydroalanine) as well as those from a scrambled sequence. The formation
of these uncommon types of product ions, likely caused by the lack of mobile protons, were proposed to involve bond rearrangements
via a six-membered ring transition state and/or salt bridge(s). A search of 20 pseudo MS3 spectra against the Gallus gallus (chicken) database using Batch-Tag, a program originally designed for bottom up MS/MS analysis,
identified chicken lysozyme as the only hit with the expectation values less than 0.02 for 12 of the spectra. The pseudo MS3 approach may help to identify disulfide-bonded proteins and determine the associated post-translational modifications (PTMs);
the confidence in the identification may be improved by incorporating the fragmentation characteristics into currently available
search programs. 相似文献
The behaviour of sulfadiazine (SDZ) and its metabolites was investigated by administering the 14C-labelled veterinary drug to fattening pigs. The excretion kinetics were determined after daily collection of manure. Two
known metabolites, N-acetylsulfadiazine and 4-hydroxysulfadiazine, and two hitherto unidentified minor metabolites were recovered. Various mass
spectrometric techniques such as parent, product ion scans and accurate mass measurement were used. The new compounds were
identified as N-formylsulfadiazine (For-SDZ) and N-acetyl-4-hydroxysulfadiazine (Ac-4-OH-SDZ). The identification of SDZ, Ac-SDZ and For-SDZ was confirmed by comparison of
the spectroscopic and chromatographic data of the synthesized authentic references. The identification of the hydroxylated
compounds 4-OH-SDZ and Ac-4-OH-SDZ was performed by MSn, and accurate mass measurements. Only 4% of the administered radioactivity remained in the pig after ten days and SDZ accounted
for 44% of the 96% radioactivity excreted. More than 93% of the labelled compounds were detected and identified in the manure.
The key analytical problem, namely a high concentration of matrix in sample extracts, was overcome by advanced measurement
techniques and with the use of a suitable internal standard. The mean recoveries for all compounds were ≥96%. Linearity was
established over a concentration range of 0.5 to 10,000 μg kg−1 manure with a correlation coefficient ≥0.99. The same experiment was carried out simultaneously with non-labelled SDZ to
obtain manure for outdoor soil experiments. 相似文献
Direct tissue imaging was performed on dissected insect tissue using a MALDI ion trap to visualize endogenous neuropeptides. Coupling tissue imaging to tandem MSn allows for the identification of previously known species and the ability to identify new ones by de novo sequencing, as searchable databases for insects are sparse. Direct tissue imaging is an attractive technique for the study of neuropeptides as minimal sample preparation is required prior to mass spectrometry. We successfully identified neuropeptides present in the corpora cardiaca and allata of Acheta domesticus (the house cricket). Diagnostic fragments at low m/z were used to distinguish between lipids and neuropeptides. The distribution of peptides appears to be more differentially localized than that of phospholipids, which seem to be more evenly distributed within the tissue. 相似文献
Gas-phase infrared photodissociation spectroscopy is reported for the microsolvated [Mn(ClO4)(H2O)n]+ and [Mn2(ClO4)3(H2O)n]+ complexes from n = 2 to 5. Electrosprayed ions are isolated in an ion-trap where they are photodissociated. The 2600–3800 cm−1 spectral region associated with the OH stretching mode is scanned with a relatively low-power infrared table-top laser, which
is used in combination with a CO2 laser to enhance the photofragmentation yield of these strongly bound ions. Hydrogen bonding is evidenced by a relatively
broad band red-shifted from the free OH region. Band assignment based on quantum chemical calculations suggest that there
is formation of water—perchlorate hydrogen bond within the first coordination shell of high-spin Mn(II). Although the observed
spectral features are also compatible with the formation of structures with double-acceptor water in the second shell, these
structures are found relatively high in energy compared with structures with all water directly bound to manganese. Using
the highly intense IR beam of the free electron laser CLIO in the 800–1700 cm−1, we were also able to characterize the coordination mode (η2) of perchlorate for two clusters. The comparison of experimental and calculated spectra suggests that the perchlorate Cl—O
stretches are unexpectedly underestimated at the B3LYP level, while they are correctly described at the MP2 level allowing
for spectral assignment. 相似文献
Infusion-based electrospray ionization (ESI) coupled to multiple-stage tandem mass spectrometry (MSn) is a standard methodology for investigating lipid A structural diversity (Shaffer et al. J. Am. Soc. Mass. Spectrom. 18(6),
1080–1092, 2007). Annotation of these MSn spectra, however, has remained a manual, expert-driven process. In order to keep up with the data acquisition rates of modern
instruments, we devised a computational method to annotate lipid A MSn spectra rapidly and automatically, which we refer to as hierarchical tandem mass spectrometry (HiTMS) algorithm. As a first-pass
tool, HiTMS aids expert interpretation of lipid A MSn data by providing the analyst with a set of candidate structures that may then be confirmed or rejected. HiTMS deciphers
the signature ions (e.g., A-, Y-, and Z-type ions) and neutral losses of MSn spectra using a species-specific library based on general prior structural knowledge of the given lipid A species under investigation.
Candidates are selected by calculating the correlation between theoretical and acquired MSn spectra. At a false discovery rate of less than 0.01, HiTMS correctly assigned 85% of the structures in a library of 133
manually annotated Francisella tularensis subspecies novicida lipid A structures. Additionally, HiTMS correctly assigned 85% of the structures in a smaller library of lipid A species
from Yersinia pestis demonstrating that it may be used across species. 相似文献
Structure elucidation of steroids by mass spectrometry has been of great importance to various analytical arenas and numerous
studies were conducted to provide evidence for the composition and origin of (tandem) mass spectrometry-derived product ions
used to characterize and identify steroidal substances. The common product ion at m/z 97 generated from androst-4-ene-3-one analogs has been subject of various studies, including stable isotope-labeling and
(high resolution/high accuracy) tandem mass spectrometry, but its gas-phase structure has never been confirmed. Using high
resolution/high accuracy mass spectrometry and low resolution tandem mass spectrometry, density functional theory (DFT) calculation,
and infrared multiple photon dissociation (IRMPD) spectroscopy employing a free electron laser, the structure of m/z 97 derived from testosterone was assigned to protonated 3-methyl-2-cyclopenten-1-one. This ion was identified in a set of
six cyclic C6H9O+ isomers as computed at the B3LYP/6-311++G(2d,2p) level of theory (protonated 3-methyl-2-cyclopenten-1-one, 2-methyl-2-cyclopenten-1-one
and 2-cyclohexen-1-one). Product ions of m/z 97 obtained from MS2 and MS3 experiments of protonated 3-methyl-2-cyclopenten-1-one, 2-methyl-2-cyclopenten-1-one, 2-cyclohexen-1-one, and testosterone
corroborated the suggested gas-phase ion structure, which was eventually substantiated by IRMPD spectroscopy yielding a spectrum
that convincingly matched the predicted counterpart. Finally, the dissociation pathway of the protonated molecule of testosterone
to m/z 97 was revisited and an alternative pathway was suggested that considers the exclusion of C-10 along with the inclusion of
C-5, which was experimentally demonstrated with stable isotope labeling. 相似文献
The rapid separation of isomeric precursor ions of oligosaccharides prior to their analysis by mass spectrometry to the nth power (MSn) was demonstrated using an ambient pressure ion mobility spectrometer (IMS) interfaced with a quadrupole ion trap. Separations
were not limited to specific types of isomers; representative isomers differing solely in the stereochemistry of sugars, in
their anomeric configurations, and in their overall branching patterns and linkage positions could be resolved in the millisecond
time frame. Physical separation of precursor ions permitted independent mass spectra of individual oligosaccharide isomers
to be acquired to at least MS3, the number of stages of dissociation limited only practically by the abundance of specific product ions. IMS–MSn analysis was particularly valuable in the evaluation of isomeric oligosaccharides that yielded identical sets of product
ions in tandem mass spectrometry experiments, revealing pairs of isomers that would otherwise not be known to be present in
a mixture if evaluated solely by MS dissociation methods alone. A practical example of IMS–MSn analysis of a set of isomers included within a single high-performance liquid chromatography fraction of oligosaccharides
released from bovine submaxillary mucin is described. 相似文献
A sequential separation procedure has been developed for the determination of 99Tc, 94Nb, 55Fe, 90Sr and 59/63Ni in various radioactive wastes generated from nuclear power plants. Ion exchange and extraction chromatography were adopted
for individual separation of the radionuclides. Precipitation was supplementarily utilized for both purification of the individual
radionuclides and preparation of the radionuclide sources for use in a radioactivity measurement. The chromatographic separation
behavior of the radionuclides both from the sample matrix metals and from one another was investigated using stable metals,
Re (as a surrogate of 99Tc), Nb, Fe, Sr and Ni. The validity of the procedure for reliability and applicability was evaluated by measuring the recovery
of the metal carriers added to synthetic radioactive waste solutions. The recoveries by the chromatographic separation were
in the range of 84.8 to 102.2% with 2s of less than 8.6%, the recoveries by the precipitation being in the range of 84.3 to 97.3% with 2s of less than 10.9%. 相似文献
Dissociative electron ionization of diethyl dithiophosphate (I) and O,O′-diethyl methylphosphonothioate (II) generates moderately abundant m/z 81 ions of composition [P, O, S, H2]+. From tandem mass spectrometry experiments and theoretical calculations at the B3LYP/6-31G(d,p), G2, and G2 (MP2) levels
it is concluded that the majority of the ions have the structure of HS-P-OH+ (1a+) and it is separated by high-energy barriers from its isomers P(= S)OH2+ (1b+), P(= O)SH2+ (1c+), HP(= S)OH+ (1d+), and HP(= O)SH+ (1e+). Low-energy (metastable) ions 1a+ dissociate via losses of H2O and H2S to yield m/z 63 (PS+) and m/z 47 (PO+) product ions, respectively. These reactions involve isomerization of 1a+ into the stable isomers 1b+ and 1c+. Neutralization-reionization experiments confirm the theoretical prediction that radical 1a· is a stable species in the gas-phase. Variable-time NR experiments indicated that only a small fraction of metastable 1a· radicals dissociate in the 0.4–4.6 μs time window, while most dissociations occurred on a shorter time scale. RRKM calculations were performed to investigate
unimolecular dissociation kinetics of 1a· which were found to be in agreement with the fragmentation observed in the NR spectrum. The 70-eV electron ionization of
(I) and diethyl chlorothiophosphate (III) yields m/z 97 ions, predominantly of the structure S = P(OH)2+ (2a+). This conclusion follows from tandem mass spectrometry experiments and theoretical calculations. The calculations predict
that (2a+) is separated by high-energy barriers from its isomers O = P(SH)OH+ (2b+), S = P(= O)OH2+ (2c+), and O = P(= O)SH2+ (2d+). Neutralization-reionization experiments confirmed that 2a· radical is a kinetically stable species on the time scale of up to 5 μs, which is in agreement with ab initio calculations. However, owing to a mismatch of Franck-Condon factors a large fraction
of 2a· dissociates by loss of SH· yielding O=P-OH. 相似文献
