Internal energies and energy distributions were studied using the 'survival yield' method developed previously. In addition to conventional benzylpyridinium salts, protonated esters (fragmenting by rearrangement) and protonated leucine enkephalin were also used, extending the validity of the technique. Fragmentation processes were studied in the cone voltage region and modeled by the RRKM-based MassKinetics program. The results show that the shapes of the energy distributions are similar to thermal distributions. The mean internal energies are very similar for all compound classes studied, and show a linear increase with collision energy in the 10-50 eV region.
The yield of metallation of methionine-enkephalin and leucine-enkephalin isomers by copper(II) chloride was investigated by electrospray ionization ion trap mass spectrometry (ESI-ITMS) in negative ionization mode. Binary ([(M-3H)+Cu(II)](-)) and ternary ([(M-3H)+Cu(II)Cl](-)) complexes were observed. Soft and hard desolvation conditions (by changing the declustering voltage) were applied to study their influence on the metallation yield and on the observed deprotonated and metallated species. Structures of the binary complexes with defined charge locations are proposed, based on the observed in-source fragmentations. It was demonstrated that the in-source fragmentations under hard desolvation conditions could differentiate the Leu/Ile isomers if located at the C-terminal position but not at the N-terminal position. This behavior was also observed using a triple quadrupole analyzer. This facile distinction, due to a different radical loss from the [(M-3Hbond;CO(2))+Cu(II)](-) species (loss of [C(3)H(7)](.) for YGGFL and [C(2)H(5)](.) for YGGFI), was facilitated by the reduction of the oxidation state of Cu(II). This in-source differentiation of YGGFI and YGGFL was also implemented in LC/ESI-MS analysis by post-column addition of the copper salt with a syringe pump.
Preconcentration of nerve agent degradation products (alkyl methylphosphonic acids) contained in high-conductivity matrices was performed using transient ITP to enhance sensitivity of CE-ESI-MS. The separation conditions of the five studied alkyl methylphosphonic acids in CE-MS were first optimized. The presence of methanol in the separation medium was required to obtain a good separation of the analytes under counter-EOF conditions. Preconcentration by ITP was induced by the BGE acting as leading electrolyte (LE) while the terminating electrolyte (TE) was loaded before the sample because of the counter-EOF conditions. Different leading ions (formate or acetate) and LE concentrations were tested. The best results for the analysis of soil extracts fortified with the analytes were obtained with an LE composed of 30 mM CH(3)COONH(4) adjusted to pH 8.8 with ammonium hydroxide in (35:65 v/v) MeOH/H(2)O mixture. The TE consisted of 200 mM glycine adjusted to pH 10.0 with ammonium hydroxide in the same solvent mixture. The loading length of the TE zone was optimized. The initial pH of the TE, which determined the initial mobility of the terminating ion, appeared to markedly influence the resolution and the sensitivity. This transient ITP-CZE-MS method was then adapted for the analysis of rat urine samples fortified with the analytes, which required the use of a more concentrated LE (50 mM). LODs between 4 and 70 ng/mL in soil extract, and between 5 and 75 ng/mL in rat urine were reached from extracted ion electropherograms.
Peptide metallation with Cu2+ was explored in the negative ESI mode using an ion trap mass spectrometer. Under these conditions, the [(M-3H) + CuII]- species formed were investigated under low-energy collision-induced dissociation conditions. MS2 experiments indicate a very different behavior of CuII metallated complexes compared with [M-H]- species. CuII induces an easy loss of CO2 and specific side-chain cleavages (by radical losses) at the C-terminal residue, as observed previously by prompt 'in source' dissociation experiments. The loss of CO2 yields an unstable carbylide that leads to further dissociations involving the migration of a proton or a hydrogen radical (through the reduction of CuII). Multistage MS3 experiments were carried out to rationalize this behavior. Fragmentation pathways are proposed in order to explain the product ions observed. The side-chain radical loss at the C-terminus was demonstrated to be a consecutive process. Finally, evidence is provided that the specific side-chain cleavages can be used for the differentiation of Leu/Ile and Gln/Lys residues when they are located at the C-terminus. The existence of a zwitterionic form in the case of the anionic YGGFK-CuII complex is proposed.
Human butyrylcholinesterase is a serine hydrolase that reacts with organophosphorus compounds (OP) to form stable adducts. These adducts are valuable biomarkers for OP exposure and can be analyzed by liquid chromatography-tandem mass spectrometry (LC-MS/MS) after a preliminary digestion step in solution. However, this digestion step is time-consuming and cannot be directly coupled with LC-MS set ups. Therefore, the aim of this work was to develop pepsin-based immobilized enzyme microreactors (IMERs) for the rapid digestion of human butyrylcholinesterase (HuBuChE). Various IMERs were synthesized by grafting different amounts of pepsin on a CNBr-sepharose gel and the grafting yield was measured by a bicinchoninic acid assay (BCA). A sensitive nanoLC-MS/MS method was developed to evaluate the digestion yields of HuBuChE on IMERs which was made possible by a synthetic peptide which was used as a calibrant. The digestion was optimized by studying the impact of different parameters such as the digestion time, the temperature and the amount of pepsin grafted on IMER. This optimization allowed HuBuChE to be digested with-in 20min without pretreatment and with digestion yields up to 20%. The repeatability of the IMER synthesis and HuBuChE digestion was highlighted with the characterization of 3 similar IMERs. Finally, the digestion yields of HuBuChE were higher with IMERs when compared to a typical in solution digestion.
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