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High performance liquid chromatography mass transfer

A different strategy has been applied in our work, that emphasizes the importance of DNA stability on hole transfer within double-stranded DNA. This work is based on determination of the overall yield of oxidized nucleosides that arise from the conversion of initially generated purine and pyrimidine radical cations within DNA exposed to two-photon UVC laser pulses. On the one hand, this work benefits from the excellent current knowledge of chemical reactions involving the radical cations of DNA bases, and on the other hand, from major analytical improvements that include recent availability of the powerful technique of high performance liquid chromatography-electrospray ionization-tandem mass spectrometry (CLHP-ESI-MS/MS) [16-18]. [Pg.13]

Particulate sorbents are available almost exclusively in the shape of micrometersized beads. These beads are packed in columns and represent currently the most common stationary phases for high-performance liquid chromatography (HPLC). Despite their immense popularity, slow diffusional mass transfer of macromolecular solutes into the stagnant pool of the mobile phase present in the pores of the separation medium and the large void volume between the packed particles are considered to be major problems in the HPLC of macromolecules, frequently impairing their rapid and efficient separation [1]. [Pg.89]

Currently, high-performance liquid chromatography (HPLC) combined with atmospheric pressure ionization (API) triple-quadrupole mass spectrometry (MS) is the predominate quantitative technique used in modem pharmaceutical bioanalysis. The key technological achievement in API-MS was the efficient ionization in a liquid stream and transference of ions from atmosphere to vacuum. Of the API approaches developed, electrospray ionization (ESI) is the most commonly used. ESI provides an efficient means of soft ionization amenable to most molecules encountered in a dmg discovery setting. An alternative soft ionization approach is the use of desorption ionization (DI) techniques. The major distinguishing feature of DI techniques is that ions are typically produced from dried samples. [Pg.342]

Mass spectrometry (MS) is one of the most powerful detection techniques used in liquid-phase analyses,1 mainly due to the ease of interfacing with separation techniques such as capillary electrophoresis (CE)2,3 and high-performance liquid chromatography (HPLC).4 Due to its sensitivity and applicability to a wide variety of chemical and biochemical species, MS is also used for the analysis of (bio)chemical molecules processed in microfluidics devices.5,6 Electrospray ionization (ESI)7 10 is often used to transfer samples from microfluidics chips to a mass spectrometer, involving analyte ionization directly from solutions and operating at flow rates typically used in microfluidics devices.11 Due to its effectiveness, the use of chip-MS coupling has rapidly spread in many research areas with bioanalytical applications,12 such as the... [Pg.201]


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