Glutathione peroxidase (isolated from bovine erythrocytes) and its behaviour during alkylation and enzymatic digestion were
studied by various hyphenated techniques: gel electrophoresis–laser ablation (LA) inductively coupled plasma (ICP) mass spectrometry
(MS), size-exclusion liquid chromatography–ICP MS, capillary high-performance liquid chromatography (capHPLC)–ICP MS, matrix-assisted
laser desorption/ionization (MALDI) time-of-flight (TOF) MS, electrospray MS, and nanoHPLC–electrospray ionization (ESI) MS/MS.
ESI TOF MS and MALDI TOF MS allowed the determination of the molecular mass but could not confirm the presence of selenium
in the protein. The purity of the protein with respect to selenium species could be evaluated by LA ICP MS and size-exclusion
chromatography (SEC)–ICP MS under denaturating and nondenaturating conditions, respectively. SEC–ICP MS and capHPLC–ICP MS
turned out to be valuable techniques to study the enzymolysis efficiency, miscleavage and artefact formation during derivatization
and tryptic digestion. For the first time the parallel ICP MS and ESI MS/MS data are reported for the selenocysteine-containing
peptide extracted from the gel; capHPLC–ICP MS allowed the sensitive detection of the selenopeptide regardless of the matrix
and nanoHPLC–electrospray made possible its identification.
Figure Eye catching image
Electronic supplementary material The online version of this article (doi:) contains supplementary material, which is available to authorized users. 相似文献
In a clinical diagnosis microbiology laboratory, the current method of identifying bacterial isolates is based mainly on phenotypic
characteristics, for example growth pattern on different media, colony morphology, Gram stain, and various biochemical reactions.
These techniques collectively enable great accuracy in identifying most bacterial isolates, but are costly and time-consuming.
In our clinical microbiology laboratory, we prospectively assessed the ability of matrix-assisted laser desorption ionization–time
of flight mass spectrometry (MALDI–TOF MS) to identify bacterial strains that were routinely isolated from clinical samples.
Bacterial colonies obtained from a total of 468 strains of 92 bacterial species isolated at the Department of Clinical Laboratory
at Chiba University were directly placed on target MALDI plates followed by addition of CHCA matrix solution. The plates were
then subjected to MALDI–TOF MS measurement and the microorganisms were identified by pattern matching with the libraries in
the BioTyper 2.0 software. Identification success at the species and genus levels was 91.7% (429/468) and 97.0% (454/468),
respectively. MALDI–TOF MS is a rapid, simple, and high-throughput proteomic technique for identification of a variety of
bacterial species. Because colony-to-colony differences and effects of culture duration on the results are minimal, it can
be implemented in a conventional laboratory setting. Although for some pathogens, preanalytical processes should be refined,
and the current database should be improved to obtain more accurate results, the MALDI–TOF MS based method performs, in general,
as well as conventional methods and is a promising technology in clinical laboratories. 相似文献
A method based on ICP collision-cell MS detection in capillary HPLC was developed to gain an insight into the purity and identity of selenium-containing proteins separated by 1-D and 2-D electrophoresis. The bands and spots obtained after the separation of water-soluble proteins in selenized yeast were digested with trypsin prior to chromatography. Selenium could be detected down to the subpicogram level. The method, assisted by information obtained by MALDI TOF MS on the 5000 Da cut-off fraction, permitted the purity of bands and spots to be estimated and the efficiency of tryptic digestion and the quantity of selenium present in individual peptides to be evaluated. Owing to the high sensitivity and the lack of matrix suppression effects, the method provided chromatograms with signal-to-noise ratios of 10–1000 in conditions where the common ES Q–TOF MS detection failed.
相似文献
The ability of MALDI TOF MS (matrix-assisted laser desorption ionisation time-of-flight mass spectrometry) to identify cultivable microflora from two waste disposal sites from non-ferrous metal industry was analysed. Despite the harsh conditions (extreme pH values and heavy metal content in red mud disposal site from aluminium production or high heavy metal content in nickel sludge), relatively high numbers of bacteria were recovered. In both environments, the bacterial community was dominated by Gram-positive bacteria, especially by actinobacteria. High-quality MALDI TOF mass spectra were obtained but most of the bacteria isolates could be not identified using MALDI Biotyper software. The overall identification rate was lower than 20 %; in two of the environments tested identification rates were lower than 10 %. As a dominant bacterial species, Microbacterium spp. in drainage water from an aluminium red mud disposal site near ?iar nad Hronom, Bacillus spp. in red mud samples from the same site, and Arthrobacter spp. from nickel smelter sludge near Sereï were identified by a combination of the Biolog system and 16S rRNA sequence analysis. As the primary focus of the MALDI TOF MS-based methodology is directed towards medically important bacteria, reference database spectra expansion and refinement are needed to improve the ability of MALDI TOF MS to identify environmental bacteria, especially those from extreme environments. 相似文献
After completion of the human genome sequence the search for differences among individual genomes has become the centre of
focus for geneticists. Two different types of polymorphism—single nucleotide polymorphisms (SNPs) and short tandem repeats
(STRs)—are major sources of genetic diversity and are of widespread use in genetic analysis. A plethora of genotyping techniques
have been developed, and mass spectrometry (MS) is among the most widely used analytical platforms. The most striking advantage
of mass spectrometric genotyping assays over others is the use of the measured molecular mass information for allele calling.
The molecular mass is less error-prone than other sequence-specific parameters, including migration times, retention times,
or hybridization yields, as it represents an intrinsic property of a nucleic acid molecule that is directly related to its
nucleotide composition. Mass spectrometric assays can roughly be divided into two major groups—matrix-assisted laser desorption/ionization
(MALDI)-based and electrospray ionization (ESI)-based assays. An important subdivision of ESI-based genotyping methods are
approaches that originate from the hyphenation of liquid chromatography (LC) to MS. The principles of these three classes
of mass spectrometric genotyping techniques are summarized in this review. Possibilities and limitations are critically discussed
to assist scientists, especially non-experts in MS, in choosing the appropriate mass spectrometric assay for genotyping a
genetic marker of interest.
Figure Comparison of the principle workflows applied for the characterization of genetic markers by MALDI–MS, ESI–MS, and LC–MS 相似文献
Matrix-assisted laser desorption/ionization (MALDI) mass spectrometry (MS) has been used for the discovery of hundreds of novel cell to cell signaling peptides. Beyond its advantages of sensitivity and minimal sample preparation requirements, MALDI MS is attractive for biological analyses as high quality mass spectra may be obtained directly from specific locations within prepared tissue sections. However, due to the large quantity of salts present in physiological tissues, these mass spectra often contain many adducts of cationic salts such as sodium and potassium, in addition to the molecular ion [M + H]+. To reduce the presence of cation adducts in MALDI mass spectra obtained directly from tissues, we present a methodology that uses a slow condensation procedure to enable the formation of distinct regions of matrix/analyte crystals and cation (salt) crystals. Secondary ion mass spectrometric imaging suggests that the salts and MALDI matrix undergo a mutually exclusive crystallization process that results in the separation of the salts and matrix in the sample. 相似文献
Evodiamine and rutecarpine are two kinds of indole alkaloids contained in the fruit of Evodiae fructus, which have been shown to exhibit various bioactivities in humans. A liquid chromatography–tandem mass spectrometric method
(LC–MS/MS) was developed for the determination of evodiamine and rutecarpine in human serum. The serum was extracted by solid-phase
extraction (SPE) and analyzed using a C18 column and a mobile phase consisting of methanol–water (85:15) solution containing
5 mmol/L ammonium formate at a flow rate of 0.5 mL/min. The mass spectrometer was operated in positive mode, employing the
extracted ion chromatogram (EIC) for detection and quantitation of evodiamine (m/z 288) and rutecarpine (m/z 304). Good linear relationships between the peak area and the concentration were obtained in the ranges of 5.2–1040 ng/mL
and 10.2–1020 ng/mL, with correlation coefficients (r) of 0.999 and 0.998, for evodiamine and rutecarpine, respectively. The repeatabilities (RSD, n=6) of quantitation for evodiamine and rutecarpine were 2.18–4.00% and 2.99–5.67%, respectively, and the recovery ranged from
90.5% to 98.1%. A comparative study of the different ionization and quantitation modes, including ESI–MS, ESI–MS/MS, APCI–MS
and APCI–MS/MS, was also accomplished. The MS/MS fragmentation mechanism of the base peak ([M+H]+, m/z 304) of evodiamine was investigated in order to identify the analytes in more complicated body fluid samples.
相似文献
Mass spectrometry imaging of lipids using MALDI–TOF/TOF mass spectrometers is of growing interest for chemical mapping of
organic compounds at the surface of tissue sections. Many efforts have been devoted to the best matrix choice and deposition
technique. Nevertheless, the identification of lipid species desorbed from tissue sections remains problematic. It is now
well-known that protonated, sodium- and potassium-cationized lipids are detected from biological samples, thus complicating
the data analysis. A new sample preparation method is proposed, involving the use of lithium salts in the matrix solution
in order to simplify the mass spectra with only lithium-cationized molecules instead of a mixture of various cationized species.
Five different lithium salts were tested. Among them, lithium trifluoroacetate and lithium iodide merged the different lipid
adducts into one single lithium-cationized species. An optimized sample preparation protocol demonstrated that the lithium
trifluoroacetate salt slightly increased desorption of phosphatidylcholines. Mass spectrometry images acquired on rat brain
tissue sections by adding lithium trifluoroacetate showed the best results in terms of image contrast. Moreover, more structurally
relevant fragments were generated by tandem mass spectrometry when analyzing lithium-cationized species. 相似文献
Mixtures of pollen grains of three different species (Corylus avellana, Alnus cordata, and Pinus sylvestris) were investigated by matrix-assisted laser desorption/ionization time-of-flight imaging mass spectrometry (MALDI-TOF imaging MS). The amount of pollen grains was reduced stepwise from >?10 to single pollen grains. For sample pretreatment, we modified a previously applied approach, where any additional extraction steps were omitted. Our results show that characteristic pollen MALDI mass spectra can be obtained from a single pollen grain, which is the prerequisite for a reliable pollen classification in practical applications. MALDI imaging of laterally resolved pollen grains provides additional information by reducing the complexity of the MS spectra of mixtures, where frequently peak discrimination is observed. Combined with multivariate statistical analyses, such as principal component analysis (PCA), our approach offers the chance for a fast and reliable identification of individual pollen grains by mass spectrometry.
A new type of metal-oxide-coated magnetic nanoparticles (NPs)—tantalum-oxide-coated magnetic iron oxide (Fe3O4@Ta2O5) NPs—which are used as affinity probes for selectively trapping phosphopeptides from complex samples, is demonstrated in
this study. In this approach, phosphopeptide enrichment was achieved by incubating the NPs with sample solutions under microwave
heating within 1 min. The NP–target species conjugates were readily isolated from samples by magnetic separation followed
by matrix-assisted laser desorption/ionization (MALDI) mass spectrometric analysis. When using human serum as the sample,
phosphorylated fibrinopeptide-A-derived ions are the only ions observed in the MALDI mass spectra after enrichment by the
Fe3O4@Ta2O5 NPs. Furthermore, only phosphopeptides appear in the MALDI mass spectra after using the affinity probes to selectively trap
target species from the tryptic digest of a cell lysate and milk sample. The results demonstrated that the Fe3O4@Ta2O5 NPs have the capability of selectively trapping phosphorylated peptides from complex samples. The detection limit of this
approach for a phosphopeptide (FQpSEEQQQTEDELQDK) was ~10 fmol.
Figure For the first time, tantalum oxide-coated magnetic iron oxide (Fe3O4@Ta2O5) NPs were demonstrated as suitable affinity-probes for selectively trapping phosphopeptides from complex samples. To shorten
the analysis time, phosphopeptide enrichment was achieved by incubating the NPs with sample solutions under microwave-heating
within 1 min. MALDI MS was employed for characterization of the species trapped by the NPs. 相似文献
Direct methylation and solid-phase microextraction (SPME) were used as a sample preparation technique for classification of
bacteria based on fatty acid methyl ester (FAME) profiles. Methanolic tetramethylammonium hydroxide was applied as a dual-function
reagent to saponify and derivatize whole-cell bacterial fatty acids into FAMEs in one step, and SPME was used to extract the
bacterial FAMEs from the headspace. Compared with traditional alkaline saponification and sample preparation using liquid–liquid
extraction, the method presented in this work avoids using comparatively large amounts of inorganic and organic solvents and
greatly decreases the sample preparation time as well. Characteristic gas chromatography/mass spectrometry (GC/MS) of FAME
profiles was achieved for six bacterial species. The difference between Gram-positive and Gram-negative bacteria was clearly
visualized with the application of principal component analysis of the GC/MS data of bacterial FAMEs. A cross-validation study
using ten bootstrap Latin partitions and the fuzzy rule building expert system demonstrated 87 ± 3% correct classification
efficiency.
相似文献
Matrix-assisted laser desorption ionization (MALDI) time-of-flight mass spectrometry (TOF MS) is now accepted as a quick, easy-to-use, cost-effective, and accurate technique for the identification of microorganisms. However, the successful identification of microorganisms is dependent upon careful attention to factors such as growth conditions, extraction methods, mass spectral data collection, and data analysis procedures. Currently, most microorganism identification has been limited to the species level, and only a limited number of publications have been successful in achieving strain-level identification. In this work, a “cell-free” approach is introduced where peptide analytes secreted by several Saccharomyces cerevisiae strains during their growth period are analyzed. The analysis of the cell supernatant generates mass spectral patterns that are specific to each strain. The patterns generated in combination with a robust data analysis workflow using the open-source programs MALDIquant and Mass-Up allows for strain-level identification of S. cerevisiae. The cell-free approach using the yeast supernatant to accurately identify yeast strains is presented here as a proof of concept.
Despite the worldwide existing regulation banning the use of the recombinant equine growth hormone (reGH) as growth promoter,
it is suspected to be used in horseracing to improve performances. Various analytical methods previously developed to screen
for its misuse have encountered some limitations in terms of detection timeframes, in particular during the first days following
reGH administration. A novel strategy involving the characterization of global metabolomic fingerprints in urine samples of
non-treated and reGH-treated horses by liquid chromatography–electrospray–high-resolution mass spectrometry (LC-ESI-HRMS)
is described and assessed in this paper in order to develop a new screening tool for growth hormone abuse in horseracing.
The strategy involves a limited sample preparation of the urine samples and the use of appropriate software for data processing
and analysis. As preliminary work, reproducibility of both sample preparation and mass spectrometry (MS) measurements was
evaluated in order to demonstrate the reliability of the method. Application of the developed protocol on two horses demonstrated
the suitability of the developed strategy and preliminary results showed significant modifications of the metabolome after
treatment with reGH.
相似文献
In the present study a headspace solid-phase dynamic extraction method coupled to gas chromatography–mass spectrometry (HS-SPDE-GC/MS)
for the trace determination of volatile halogenated hydrocarbons and benzene from groundwater samples was developed and evaluated.
As target compounds, benzene as well as 11 chlorinated and brominated hydrocarbons (vinyl chloride, dichloromethane, cis-1,2-dichloroethylene, trans-1,2-dichloroethylene, carbon tetrachloride, chloroform, trichloroethylene, tetrachloroethylene, bromoform) of environmental
and toxicological concern were included in this study. The analytes were extracted using a SPDE needle device, coated with
a poly(dimethylsiloxane) with 10% embedded activated carbon phase (50-μm film thickness and 56-mm film length) and were analyzed
by GC/MS in full-scan mode. Parameters that affect the extraction yield such as extraction and desorption temperature, salting-out,
extraction and desorption flow rate, extraction volume and desorption volume, the number of extraction cycles, and the pre-desorption
time have been evaluated and optimized. The linearity of the HS-SPDE-GC/MS method was established over several orders of magnitude.
Method detection limits (MDLs) for the compounds investigated ranged between 12 ng/L for cis-dichloroethylene and trans-dichloroethylene and 870 ng/L for vinyl chloride. The method was thoroughly validated, and the precision at two concentration
levels (0.1 mg/L and a concentration 5 times above the MDL) was between 3.1 and 16% for the analytes investigated. SPDE provides
high sensitivity, short sample preparation and extraction times and a high sample throughput because of full automation. Finally,
the applicability to real environmental samples is shown exemplarily for various groundwater samples from a former waste-oil
recycling facility. Groundwater from the site showed a complex contamination with chlorinated volatile organic compounds and
aromatic hydrocarbons.
Figure SPDE Principle 相似文献
Liquid chromatography (LC) hyphenated with both elemental and molecular mass spectrometry has been used for Se speciation
in Se-enriched garlic. Different species were separated by ion-pair liquid chromatography–inductively coupled plasma mass
spectrometry (LC–ICP–MS) after hot-water extraction. They were identified by on-line reversed-phase liquid chromatography–electrospray
ionization tandem mass spectrometry (RPLC–ESI–MS–MS). Se-methionine and Se-methylselenocysteine were determined by monitoring
their product ions. Another compound, γ-glutamyl-Se-methylselenocysteine, shown to be the most abundant form of Se in the
garlic, was determined without any additional sample pre-treatment after extraction and without the need for a synthesized
standard. Product ions for this dipeptide were detected by LC–ESI–MS–MS for three isotopes of Se—78Se, 80Se: and 82Se. The method was extended to the species extracted during in-vitro gastrointestinal digestion. Because both Se-methylselenocysteine
and γ-glutamyl-Se-methylselenocysteine have anticarcinogenic properties, their extractability and stability during human digestion
are very important. Garlic was also treated with saliva, to enable detection and analysis of species extracted during mastication.
Detailed information on the extractability of selenium species by both simulated gastric and intestinal fluid are given, and
variation of the distribution of Se among the different species with time is discussed. Although the main species in garlic
is the dipeptide γ-glutamyl-Se-methylselenocysteine, Se-methylselenocysteine is the main compound present in the extracts
after treatment with gastrointestinal fluids. Two more, so far unknown compounds were observed in the chromatogram. The extracted
species and their transformations were analysed by combining LC–ICP–MS and LC–ESI–MS–MS. In both the simulated gastric and
intestinal digests, Se-methionine, Se-methylselenocysteine, and γ-glutamyl-Se-methylselenocysteine could be determined by
LC–ESI–MS–MS by measuring their typical product ions.
相似文献
This paper describes a headspace solid-phase microextraction (HS-SPME) procedure coupled to gas chromatography with mass spectrometric
detection (GC–MS) for the determination of eight PAHs in aquatic species. The influence of various parameters on the PAH extraction
efficiency was carefully examined. At 75 °C and for an extraction time of 60 min, a polydimethylsiloxane–divinylbenzene (PDMS/DVB)
fiber coating was found to be most suitable. Under the optimized conditions, detection limits ranged from 8 to 450 pg g−1, depending on the compound and the sample matrix. The repeatability varied between 7 and 15% (RSD). Accuracy was tested using
the NIST SRM 1974b reference material. The method was successfully applied to different samples, and the studied PAHs were
detected in several of the samples.
Figure Headspace SPME sampling followed by GC–MS facilitates routine monitoring of PAHs in aquatic species 相似文献
