Mária Katona

In vivo, in situ tissue analysis using rapid evaporative ionization mass spectrometry

The analysis of intact biological tissues by mass spectrometry (MS) has been pursued for more than three decades. However, mass spectrometric methods have always put strong constraints on the geometry and the preparation of these samples. Even with the recent advent of ambient ionization methods, not all of these restrictions have been lifted. MS analysis of biomolecules in tissue has traditionally been achieved by desorption ionization methods including secondary ion mass spectrometry (SIMS), matrix-assisted laser desorption (MALDI), 19, 20] and desorption electrospray ionization (DESI) 5,18] methods. While desorption ionization methods are not appropriate for the analysis of vital (living) tissues, rapid thermal evaporation has the potential to establish the in situ, in vivo ionization of tissue constituents. The possible formation of organic ions from condensed-phase samples in a purely thermal process was initially proposed by Holland et al., and it was successfully demonstrated later. The rationale of rapid heating was to achieve molecular evaporation rates comparable to the rate of decomposition, which results in the formation of a considerable quantity of gaseous molecules or molecular ions. The quest for efficient thermal evaporation methods has led to the development of various thermally assisted ionization methods, including thermospray ionization. Since collisional cooling of nascent ions at higher pressure is more effective, thermal evaporation at atmospheric pressure is expected to suppress thermal decomposition. Atmospheric pressure thermal desorption ionization was demonstrated recently by the desorption of organic cations with minimal thermal degradation. 27] The present study is based on the discovery that rapid thermal evaporation of biological tissues yields gaseous molecular ions of the major tissue components, for example, phospholipids. As thermal evaporation of tissues is widely used in surgery (i.e., electrosurgery and laser surgery), it was sensible to use dedicated surgical instruments for the experiments. Combination of surgical and MS techniques also offers a possibility for in situ chemical analysis of tissue during surgery. Since the key feature of the technique is the fast evaporation of a sample, it was termed “Rapid Evaporative Ionization Mass Spectrometry” (REIMS). The tentative mechanism of ion formation is described in the Supporting Information. Electrosurgical dissection is based on the Joule heating and evaporation of tissues by an electric current. The presence of ionized water molecules during electrosurgical dissection raises the possibility of an alternative ionization mechanism involving neutral desorption and chemical ionization in the gas phase. For more details, see the Supporting Information. An electrosurgical electrode was used as an ion source coupled to a distant mass spectrometer employing a Venturi gas jet pump and 1–2 m long polytetrafluoroethylene (PTFE) tubing (Figure 1).

Analysis of biological fluids by direct combination of solid phase extraction and desorption electrospray ionization mass spectrometry.

A novel, solid phase extraction (SPE)-based sample preparation method was developed for desorption electrospray ionization (DESI) mass spectrometry. Conventional SPE sample preparation was followed by a custom elution procedure. The eluate was evaporated from the closing frit of the cartridge using a gas jet. Thus the analyte was concentrated on the surface of the frit, which is ideal for DESI analysis. Application of the above SPE protocol allowed the concentration of the analyte content of up to 1 L liquid sample into a 1 mm diameter circular spot. The sample preparation procedure can improve the overall sensitivity of the method by up to 6 orders of magnitude if the sample volume is sufficient. The device has been tested using aqueous solutions of Rhodamine 116; the limit of detection was comparable to the LOD of electrospray analysis. Methodology was tested for drug monitoring applications in human serum. Levels of Cyclosporine A were determined using a 0.1 mL serum sample. Dynamic range of the method exceeded 3 orders of magnitude; the detection limit was below the therapeutic serum concentration of the drug.

A mass spectrometry based functional assay for the quantitative assessment of ABC transporter activity

ATP-Binding Cassette (ABC) transporters are highly expressed in pharmacological barriers limiting the access of drugs to their targets. Since characterization of a compound as a transporter substrate or inhibitor bears significant consequences in drug development, there is a great need for reliable tools that enable the rapid analysis of the transport susceptibility of drugs. Here we describe a simple but very efficient high-performance liquid chromatography/mass spectrometry (HPLC/MS) assay for measuring the ABC transporter-dependent vesicular transport of compounds. In addition, we provide evidence that the requirement for sample preparation can be minimized using desorption electrospray ionization (DESI)-MS, paving the way for a direct, high-throughput investigation of drug-transporter interactions.

Selective detection of specific protein-ligand complexes by electrosonic spray-precursor ion scan tandem mass spectrometry

A novel mass spectrometric method for the selective detection of specific protein-ligand complexes is presented. The new method is based on electrosonic spray ionization of samples containing protein and ligand molecules, and mass spectrometric detection using the precursor ion scanning function on a triple quadrupole instrument. Mass-selected intact protein-ligand complex ions are subjected to fragmentation by means of collision-induced dissociation in the collision cell of the instrument, while the second mass analyzer is set to the m/z of protonated ligand ions or their alkali metal adducts. The method allows for the detection of only those ions which yield ions characteristic of the ligand molecules upon fragmentation. Since the scan range of first analyzer is set well above the m/z of the ligand ion, and the CID conditions are established to permit fragmentation of only loosely bound, noncovalent complexes, the method is specific to the detection of protein-ligand complexes under described conditions. Behavior of biologically specific and nonspecific complexes was compared under various instrumental settings. Parameters were optimized to obtain maximal selectivity for specific complexes. Specific and nonspecific complexes were found to show markedly different fragmentation characteristics, which can be a basis for selective detection of complexes with biological relevance. Preparation of specific and nonspecific complexes containing identical building blocks was attempted. Complex ions with identical stoichiometry but different origin showed the expected difference in fragmentation characteristics, which gives direct evidence for the different mechanism of specific versus nonspecific complex ion formation.

Epidemiological and molecular genetic examination in epidermolysis bullosa

Semmelweis Egyetem, Általános Orvostudományi Kar, Bôr-, Nemikórtani és Bôronkológiai Klinika, Budapest, Magyarország, Zuglói Egészségügyi Szolgálat, Gyermek Bôrgyógyászat Szakrendelés, Budapest, Magyarország, Men for Care Egészségügyi Központ, Százhalombatta, Magyarország, Egyesített Szent István és Szent László Kórház és Rendelôintézet Bôrgyógyászati Szakambulancia és Lymphoedema Rehabilitációs Osztály, Budapest, Magyarország, Department of Dermatology, University of Groningen, University Medical Center Groningen, Groningen, The Netherlands

[Neonatal lupus erythematosus: case report and review of the literature].

Neonatal lupus erythematosus (NLE) is a disease of the first few months of infancy. It is caused by anti-SSA and anti-SSB antibodies, which are products of maternal autoimmune disorders (SLE, Sjögren, rheumatoid arthritis) and can be passively transported across the placenta. The prevalence of NLE is low. The major clinical findings are cutaneous (typical annular erythematous plaques), cardiac, hepatic and hematologic alterations. Its most severe consequence is third-degree heart block, which is irreversible, requires pacemaker-implantation and responsible for the 20-30% mortality rate. Symptoms usually resolve spontaneously at age of 6-9 months in association with disappearance of maternal antibodies from the infants serum. In our case the typical cutaneous manifestations covered virtually the whole body, were present at birth, however, no conduction defects developed. The fact that the mothers sickness was not known at birth made it difficult to establish the diagnosis. The significant thrombocytopaenia, progressive skin-changes and the elevated liver function tests necessitated systemic steroid treatment.