Thin-film microextraction (TFME) is a format of solid-phase microextraction (SPME) technique which offers improvement of sensitivity without sacrificing time through the increase of available surface area and extractive phase volume. This technique offers significant advantages which make it attractive for many analytical/bioanalytical applications. This review discusses the fundamental principle of TFME and its benefits versus the rod fiber geometry of SPME, and demonstrates the agreements of the experimental data for the available TFME systems with the theoretical concept. The current configurations, coating chemistries, coating preparation methods, and applications for TFME system are reported. 相似文献
The method described in this work provides a sensitive and fast technique for investigating the primary structure of peptides with molecular weight up to 3340 amu. Usually, the metastable ion kinetic energy spectra (MIKES) and collisional activated decomposition (CAD) spectra provide complementary information for the FAB mass spectra, the MIKES and CAD spectra generally contain high-mass sequence ions. 相似文献
Label-free imaging mass spectrometry provides a new look into different research areas. Will chemical mass microscopy on a biological system move from hype to hope?
In this report, a method for in-source hydrogen/deuterium (H/D) exchange at atmospheric pressure is reported. The method was named atmospheric pressure photo ionization hydrogen/deuterium exchange mass spectrometry (APPI HDX MS). H/D exchange was performed by mixing samples dissolved in toluene with CH3OD solvent and analyzing the mixture using atmospheric pressure photo ionization mass spectrometry (APPI-MS). The APPI HDX spectra obtained with contact times between the analyte solution and methanol-OD (CH3OD) of?<?0.5 s or 1 h showed the same pattern of H/D exchange. Therefore, it was concluded that APPI HDX occurred in the source but not in the solution. The proposed method does not require a specific type of mass spectrometer and can be performed at atmospheric pressure. H/D exchange can be performed in any laboratory with a mass spectrometer and a commercial APPI source. Using this method, multiple H/D exchanges of aromatic hydrogen and/or H/D exchange of active hydrogen were observed. These results demonstrated that H/D exchange can be used to distinguish between isomers containing primary, secondary, and tertiary amines, as well as pyridine and pyrrole functional groups.
A zoom–time-of-flight mass spectrometer has been coupled to an inductively coupled plasma (ICP) ionization source. Zoom–time-of-flight mass spectrometry (zoom-TOFMS) combines two complementary types of velocity-based mass separation. Specifically, zoom-TOFMS alternates between conventional, constant-energy acceleration (CEA) TOFMS and energy-focused, constant-momentum acceleration (CMA) (zoom) TOFMS. The CMA mode provides a mass-resolution enhancement of 1.5-1.7× over CEA-TOFMS in the current, 35-cm ICP-zoom-TOFMS instrument geometry. The maximum resolving power (full-width at half-maximum) for the ICP-zoom-TOFMS instrument is 1200 for CEA-TOFMS and 1900 for CMA-TOFMS. The CMA mode yields detection limits of between 0.02 and 0.8 ppt, depending upon the repetition rate and integration time—compared with single ppt detection limits for CEA-TOFMS. Isotope-ratio precision is shot-noise limited at approximately 0.2% relative-standard deviation (RSD) for both CEA- and CMA-TOFMS at a 10 kHz repetition rate and an integration time of 3–5 min. When the repetition rate is increased to 43.5 kHz for CMA, the shot-noise limited, zoom-mode isotope-ratio precision is improved to 0.09% RSD for the same integration time.
Fragmentation of phosphorylated Tau peptides in matrix assisted laser desorption/ionization-time of flight-mass spectrometry (MALDI-TOF-MS) has been investigated.According to the post-source decay (PSD) in MALDI-TOF-MS, there are two different patterns of cleavage in phosphopeptides, which can be used to determine the phosphorylated site in peptides.In the synthetic tau peptides, the fragmentation at proline residue occurs strongly and this is useful to determine the structure of tau peptides. 相似文献
Stimulated by the interest in developing gold compounds for treating cancer, gold ion–angiotensin peptide interactions are
investigated by mass spectrometry. Under the experimental conditions used, the majority of gold ion–angiotensin peptide complexes
contain gold in the oxidation states I and III. Both ESI-MS and MALDI-TOF MS detect singly/multiply charged ions for mononuclear/multinuclear
gold-attached peptides, which are represented as [peptide + a Au(I) + b Au(III) + (e - a -3b) H]e+, where a,b ≥ 0 and e is charge. ESI-MS data shows singly/multiply charged ions of Au(I)-peptide and Au(III)-peptide complexes.
This study reveals that MALDI-TOF MS mainly detects singly charged Au(I)-peptide complexes, presumably due to the ionization
process. The electrons in the MALDI plume seem to efficiently reduce Au(III) to Au(I). MALDI also tends to enhance the higher
polymeric forms of gold-peptide complexes regardless of the laser power used. Collision-induced dissociation experiments of
the mononuclear and dinuclear gold-attached peptide ions for angiotensin peptides show that the gold ion (a soft acid) binding
sites are in the vicinity of Cys (a soft ligand), His (a major anchor of peptide for metal ion chelation), and the basic residue
Arg. Data also suggests that the abundance of gold-attached peptides increases with higher gold concentration until saturation,
after which an increase in gold ion concentration leads to the aggregation and/or precipitation of gold-bound peptides. 相似文献
The atmospheric pressure chemical ionization/time,of-flight mass speetrmtry (APEI/TOF-MS) was applied to determine the mass of five a.aIIenic alcohols via their vrotonated molecu.lar ions nslna Imsifive ion mode. Polyethylene Idycol (PEG) was used as the hlternal reference. All results were obtained under the resolution of about 5000 FWHM (full width at the half maximum). Solvent effects were studied and the satired results were obtained in acetonitrile. Comvared with the theoreflcal values, nun absolute errors were less thRn 1.0 mmu. The efTeets Of nozzle pote.Jldal, push pulse potential, pug pulse potentlai, puO bias potential and ic(lulsltion rate on exact mass determina/lon were also discussed. APCI/TOF.MS is proven to be a very semi/ire analytical technique and an alternative ionizafion mode in analytical technique lablle compounds with relatively weak polarity, such as a-allenic alcohol. 相似文献
Electrospray ionization mass spectrometry (ESI-MS) is nowadays one of the cornerstones of biomolecular mass spectrometry and proteomics. Advances in sample preparation and mass analyzers have enabled researchers to extract much more information from biological samples than just the molecular weight. In particular, relevant for structural biology, noncovalent protein–protein and protein–ligand complexes can now also be analyzed by MS. For these types of analyses, assemblies need to be retained in their native quaternary state in the gas phase. This initial small niche of biomolecular mass spectrometry, nowadays often referred to as “native MS,” has come to maturation over the last two decades, with dozens of laboratories using it to study mostly protein assemblies, but also DNA and RNA-protein assemblies, with the goal to define structure–function relationships. In this perspective, we describe the origins of and (re)define the term native MS, portraying in detail what we meant by “native MS,” when the term was coined and also describing what it does (according to us) not entail. Additionally, we describe a few examples highlighting what native MS is, showing its successes to date while illustrating the wide scope this technology has in solving complex biological questions.
Abstract Pyrolysis of electrochemically prepared BF4? doped polythiophene (PTh) by direct insertion probe and Currie point pyrolysis gas chromatography mass spectrometry techniques indicated that thermal decomposition of PTh occurs in two steps. In accordance with literature results, the first step is assigned to the loss of the dopant, and the second step to the degradation of the polymer backbone producing segments of various conjugation lengths. At elevated temperatures, detection of products such as H2S and C2H2 indicating cleavage of the thiophene (Th) ring was associated with a network structure. For the dedoped samples, a significant increase in the relative intensities of the peaks characteristic to the counter ion of the dopant, N(C4H9)4+ pointed out the inward diffusion of (C4H9)4N+ during the dedoping process. 相似文献
Distance-of-flight mass spectrometry (DOFMS) separates ions of different mass-to-charge (m/z) by the distance they travel in a given time after acceleration. Like time-of-flight mass spectrometry (TOFMS), separation and mass assignment are based on ion velocity. However, DOFMS is not a variant of TOFMS; different methods of ion focusing and detection are used. In DOFMS, ions are driven orthogonally, at the detection time, onto an array of detectors parallel to the flight path. Through the independent detection of each m/z, DOFMS can provide both wider dynamic range and increased throughput for m/z of interest compared with conventional TOFMS. The iso-mass focusing and detection of ions is achieved by constant-momentum acceleration (CMA) and a linear-field ion mirror. Improved energy focus (including turn-around) is achieved in DOFMS, but the initial spatial dispersion of ions remains unchanged upon detection. Therefore, the point-source nature of surface ionization techniques could put them at an advantage for DOFMS. To date, three types of position-sensitive detectors have been used for DOFMS: a microchannel plate with a phosphorescent screen, a focal plane camera, and an IonCCD array; advances in detector technology will likely improve DOFMS figures-of-merit. In addition, the combination of CMA with TOF detection has provided improved resolution and duty factor over a narrow m/z range (compared with conventional, single-pass TOFMS). The unique characteristics of DOFMS can enable the intact collection of large biomolecules, clusters, and organisms. DOFMS might also play a key role in achieving the long-sought goal of simultaneous MS/MS.
ABSTRACTA sensitive and selective method was developed to determine pesticides in carrots by gas chromatography–mass spectrometry following the development of an optimized extraction procedure. The method was validated for 30 organochlorine pesticides for gas chromatography with electron capture detection obtaining limit of detection from 0.18 to 0.92?µg/kg except for cis- and trans-permenthrin. Twenty-six carrot samples were analyzed and six pesticides were detected. The results compared with the accepted maximum residue levels in correlation to crop origin. 相似文献
The diagnostic value of the “ortho effect” for unknown identification by mass spectrometry is well known. Here, we report
the existence of a novel “meta effect,” which adds to the repertoire of useful mass spectrometric fragmentation mechanisms.
For example, the meta-specific elimination pathway described in this report enables unequivocal identification of meta isomers
from ortho and para isomers of carboxyanilides. The reaction follows a specific path to eliminate a molecule of meta-benzyne, from the anion produced after the initial decarboxylation of the precursor. Consequently, in the CID spectra of
carboxyanilides, a peak for the (R-CO-NH)– anion is observed only for the meta isomers. For example, the peaks observed at m/z 58, 86, 120, 128, and 170 from acetamido-, butamido-, benzamido, heptamido-, and decanamido-benzoates, respectively, were
specific only to the spectra of meta isomers. 相似文献
