同位素质谱与无机质谱分析

本文是《分析试验室》定期评述中“无机质谱分析”课题的第二篇评述文章,它增加了同位素质谱分析的内容,故将题目改为现今题目,它综述了1985年～1990年间同位素质谱和无机质谱的发展概况。其中包括同位素示踪、同位素稀释、火花源质谱、二次离子质谱、等离子体质谱等。内容以国内为主,也收集了少量代表学科先进水平的外国文献。     

Pyrolysis–gas chromatography mass spectrometry and field ionization mass spectrometry of polyquinones

Low- and high-molecular mass thermal decomposition products of five polyquinones with different linking aromatic structures have been analyzed by pyrolysis–gas chromatography and by direct (in-source) pyrolysis–field ionization mass spectrometry. The quantity of carboxyl groups present in the polymer is obtained by the amounts of carbon dioxide found by pyrolysis–gas chromatography. Assuming a radical thermal decomposition mechanism the distribution of ketoacidic and quinonoid segments along the macromolecular ladder could be estimated from the high-molecular mass products measured by pyrolysis–field ionization mass spectrometry. A random distribution of the two different segments was found for polyquinones with biphenylene and dibenzofuran subunits, while a structure built up of blocks of two or more identical segments was obtained for polyquinones with dibenzothiophene and diphenylmethane subunits. At the same time the anomalous structural moieties in the polyquinone ladders are also clarified with the help of the identification of the unexpected pyroysis products. Oxidated and bis-dibenzothiophene and bis-diphenylmethane subunits were found. The observed temperature dependence for the appearances of the thermal degradation products indicates that condensation and elimination reactions are taking place under the described pyrolysis conditions. Condensation in the ketoacidic segments forming new quinonoid segments proved to be important in the polymer which was a 100% poly(ketoacid), but negligible in the polyquinones containing ketoacidic segments up to 60%.     

Modern MALDI time‐of‐flight mass spectrometry

This paper focuses on development of time‐of‐flight (TOF) mass spectrometry in response to the invention of matrix‐assisted laser desorption/ionization (MALDI). Before this breakthrough ionization technique for nonvolatile molecules, TOF was generally considered as a useful tool for exotic studies of ion properties but was not widely applied to analytical problems. Improved TOF instruments and software that allow the full potential power of MALDI to be applied to difficult biological applications are described. A theoretical approach to the design and optimization of MALDI‐TOF instruments for particular applications is presented. Experimental data are provided that are in excellent agreement with theoretical predictions of resolving power and mass accuracy. Data on sensitivity and dynamic range using kilohertz laser rates are also summarized. These results indicate that combinations of high‐performance MALDI‐TOF and TOF‐TOF with off‐line high‐capacity separations may ultimately provide throughput and dynamic range several orders of magnitude greater than those currently available with electrospray LC‐MS and MS‐MS. Copyright © 2009 John Wiley & Sons, Ltd.     

Gas‐phase fragmentation reactions of protonated benzofuran‐ and dihydrobenzofuran‐type neolignans investigated by accurate‐mass electrospray ionization tandem mass spectrometry

We have investigated gas‐phase fragmentation reactions of protonated benzofuran neolignans (BNs) and dihydrobenzofuran neolignans (DBNs) by accurate‐mass electrospray ionization tandem and multiple‐stage (MSⁿ) mass spectrometry combined with thermochemical data estimated by Computational Chemistry. Most of the protonated compounds fragment into product ions B ([M + H–MeOH]⁺), C ([ B –MeOH]⁺), D ([ C –CO]⁺), and E ([ D –CO]⁺) upon collision‐induced dissociation (CID). However, we identified a series of diagnostic ions and associated them with specific structural features. In the case of compounds displaying an acetoxy group at C‐4, product ion C produces diagnostic ions K ([ C –C₂H₂O]⁺), L ([ K –CO]⁺), and P ([ L –CO]⁺). Formation of product ions H ([ D –H₂O]⁺) and M ([ H –CO]⁺) is associated with the hydroxyl group at C‐3 and C‐3′, whereas product ions N ([ D –MeOH]⁺) and O ([ N –MeOH]⁺) indicate a methoxyl group at the same positions. Finally, product ions F ([ A –C₂H₂O]⁺), Q ([ A –C₃H₆O₂]⁺), I ([ A –C₆H₆O]⁺), and J ([ I –MeOH]⁺) for DBNs and product ion G ([ B –C₂H₂O]⁺) for BNs diagnose a saturated bond between C‐7′ and C‐8′. We used these structure‐fragmentation relationships in combination with deuterium exchange experiments, MSⁿ data, and Computational Chemistry to elucidate the gas‐phase fragmentation pathways of these compounds. These results could help to elucidate DBN and BN metabolites in in vivo and in vitro studies on the basis of electrospray ionization ESI‐CID‐MS/MS data only.     

Molecular mass distributions of star‐branched polycondensates

Of late much attention has been paid to star‐branched polymers, being a good reference model for branched polymers, in general. Usually, monodisperse or narrow disperse polymers are analysed. Knowledge of molecular mass distributions is a key factor in the analysis and study of these systems. Star‐branched polycondensates can be synthesised by reaction of a difunctional ( AB ) monomer with a compound RA _f . Weight and number molecular mass distributions of star‐branched polycondensates have been studied in relation to the initial molar ratio between R and the AB monomer (α), the average molecular mass per arm (β) and the number of arms (f ). Simple probability density functions can be derived at, if molecules are split into – R (without core R ) and + R (with core R ). This enables further the representation in molecular mass units next to the representation in monomer units. Proper choice of α, β and f can either give narrower or broader distributions compared to the most probable distribution, which is the theoretical distribution for the pure AB polymer (α = 0). The resulting polymer might either have a uni‐modal or a bi‐modal molecular mass distribution.     

Glycerophospholipid profiling by high‐performance liquid chromatography/mass spectrometry using exact mass measurements and multi‐stage mass spectrometric fragmentation experiments in parallel

A profiling method for glycerophospholipids (GPs) in biological samples was developed using reversed‐phase high‐performance liquid chromatography (RP‐HPLC) coupled to hybrid linear ion trap‐Fourier transform ion cyclotron resonance mass spectrometry (LIT‐FTICRMS) with electrospray ionization (ESI) in the negative ionization mode. The method allowed qualitative (identification and structure elucidation) and relative quantitative determination of various classes of GPs including phosphatidylcholines, phosphatidylethanolamines, phosphatidylinositols, phosphatidylserines, phosphatidic acids, phosphatidylglycerols, and cardiolipins in a single experiment. Chromatographic separation was optimized by the examination of different buffer systems and special emphasis was paid on the detection by ESI‐MS. The hybrid LIT‐FTICRMS system was operated in the data‐dependent mode, switching automatically between FTICRMS survey scans and LIT‐MS/MS experiments. Thereby, exact masses for elemental composition determination and fragmentation data for identification and assignment of fatty acid residues are provided at the same time. The low absolute instrumental limits of detection (0.05 pmol for phosphatidylglycerol to 1 pmol for phosphatidic acid) complemented by a linear dynamic range of 1.5 to 2.5 orders of magnitude facilitated the relative quantification of GP species in a lipid extract from Saccharomyces cerevisiae. The developed method is a valuable tool for in‐depth GP profiling of biological systems. Copyright © 2009 John Wiley & Sons, Ltd.     

Field-ionization mass spectrometry—fragmentation and metastables

Field-ionization (FI) mass spectrometry is an established method for obtaining abundant molecular ions¹ of a variety of compounds, and recently has been used in conjunction with exact mass measurements for determination of elemental compositions of molecules.^2,3 Very little, however, has been reported on the value of normal fragment ions and metastable ions appearing in the FI spectrum as a source of structural information.     

Analysis of acrylamide in different foodstuffs using liquid chromatography–tandem mass spectrometry and gas chromatography–tandem mass spectrometry

Acrylamide levels over a wide range of different food products were analysed using both liquid chromatography–tandem mass spectrometry (HPLC–MS–MS) and gas chromatography–tandem mass spectrometry (GC–MS–MS). Two different sample preparation methods for HPLC–MS–MS analysis were developed and optimised with respect to a high sample throughput on the one hand, and a robust and reliable analysis of difficult matrices on the other hand. The first method is applicable to various foods like potato chips, French fries, cereals, bread, and roasted coffee, allowing the analysis of up to 60 samples per technician and day. The second preparation method is not as simple and fast but enables analysis of difficult matrices like cacao, soluble coffee, molasses, or malt. In addition, this method produces extracts which are also well suited for GC–MS–MS analysis. GC–MS–MS has proven to be a sensitive and selective method offering two transitions for acrylamide even at low levels up to 1 μg kg⁻¹. For the respective methods the repeatability (n=10), given as coefficient of variation, ranged from 3% (acrylamide content of 550 μg kg⁻¹) to 12% (acrylamide content of 8 μg kg⁻¹) depending on the food matrix. The repeatability (n=3) for different food samples spiked with acrylamide (5–1500 μg kg⁻¹) ranged from 1 to 20% depending on the spiking level and the food matrix. The limit of quantification (referred to a signal-to-noise ratio of 9:1) was 30 μg kg⁻¹ for HPLC–MS–MS and 5 μg kg⁻¹ for GC–MS–MS. It could be demonstrated that measurement uncertainties were not only a result of analytical variability but also of inhomogeneity and stability of the acrylamide in food.     

Optimal single‐embryo mass spectrometry fingerprinting

In pre‐implantation embryos, lipids play key roles in determining viability, cryopreservation and implantation properties, but often their analysis is analytically challenging because of the few picograms of analytes present in each of them. Matrix‐assisted laser desorption/ionization mass spectrometry (MALDI‐MS) allows obtaining individual phospholipid profiles of these microscopic organisms. This technique is sensitive enough to enable analysis of individual intact embryos and monitoring the changes in membrane lipid composition in the early stages of development serving as screening method for studies of biology and biotechnologies of reproduction. This article introduces an improved, more comprehensive MALDI‐MS lipid fingerprinting approach that considerably increases the lipid information obtained from a single embryo. Using bovine embryos as a biological model, we have also tested optimal sample storage and handling conditions before the MALDI‐MS analysis. Improved information at the molecular level is provided by the use of a binary matrix that enables phosphatidylcholines, sphingomyelins, phosphatidylserines, phosphatidylinositols and phosphoethanolamines to be detected via MALDI(±)‐MS in both the positive and negative ion modes. An optimal MALDI‐MS protocol for lipidomic monitoring of a single intact embryo is therefore reported with potential applications in human and animal reproduction, cell development and stem cell research. Copyright © 2013 John Wiley & Sons, Ltd.     

Rapid mass spectral fingerprinting of complex mixtures of decomposed lignin: Data‐processing methods for high‐resolution full‐scan mass spectra

Lignin is the second most abundant natural biopolymer and its wastes are significant sources for renewable chemicals as an alternative to conventional fossil fuels. Consequently, chemical characterization methods are required to assess the content of valuable chemicals contained in these complex lignin wastes. This short overview summarizes rapid data‐processing methods developed in our laboratory for application to full‐scan raw data from high‐resolution mass spectrometry experiments of decomposed lignin samples. The discussed graphical and statistical methods support the initial classification and elucidation of the main structural features of the lignin components without the need for time‐consuming tandem mass spectrometry analyses.