Strongest Pill Ever - Ipertrofia Prostatica Cura Con Cialis
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Strongest Pill Ever - Ipertrofia Prostatica Cura Con Cialis
Enhancement of high mass sensitivity on the Bruker UltraFlextreme with FlashDetector technology using the CovalX HM2. Introduction Traditionally, MALDI-TOF instrument used microchannel plates (MCP) for ion detection. MCP’s must first generate secondary electrons which are then amplified and their sensitivity therefore decreases with increasing ion mass. Often MCP’s will also saturate when measuring complex samples. In order to reliably measure ions at these higher masses, a more sensitive detector is required. The Bruker UltraFlextreme has recently been developed featuring a FlashDetector. This type of detector does not rely upon MCP detection and therefore can be used to measure higher mass ions. Additionally a high mass detection system for high mass detection is now commercially available. In this poster, these two new ion detectors were evaluated using identical conditions and the effects of sensitivity and saturation were evaluated. Ryan Wenzel1; Young-Ho Chung2; Alexis Nazabal3 1CovalX 2Korea Insulin 150μM Methods A Bruker UltraFlextreme MALDI–TOF/TOF instrument (Bremen, Germany) was retrofitted with a novel high mass detection system (HM2; CovalX AG, Zurich, Switzerland) installed directly after the reflectron in linear mode. The HM2 is a small vacuum chamber which can mechanically move the high mass detector under vacuum in-line of the ion flight path directly in front of the FlashDetector. The CovalX high mass detector is designed using a high voltage collision dynode surface positioned in front of a secondary electron multiplier (CD-SEM). This setup allows for easy evaluation of CD-SEM to the FlashDetector within a matter of seconds on the exact same sample inside the same instrumental conditions. Comparison Analysis Bruker UltraFlextreme retrofitted with a CovalX HM2 High-Mass detector system Four different proteins covering a broad mass range (5.7kDa to 1.1MDa) were analyzed at relatively high concentrations. Multimer peaks from each are shown as examples of MALDI “plume-adducts” and are used to show the high mass sensitivity. + UltraFlextreme FlashDetector CovalX HM2 Insulin (5.7kDa) 68kDa (12-mer) 136kDa (24-mer) BSA (66kDa) 256kDa (4-mer) 462kDa (7-mer) Immunoglobulin G (150kDa) 450kDa (3-mer) 850kDa (5-mer) Immunoglobulin M (1.1MDa) barely 570kDa easily 1.1MDa Bovine Serum Albumin 20 μM UltraFlextreme Flash Detector 12Insulin UltraFlextreme Flash Detector + 4BSA CovalX HM2 CovalX HM2 + 24Insulin 7BSA Immunoglobulin G 9μM + 3IgG All analysis are preformed on the exact same sample spots, using the exact same experimental conditions (voltages, laser, # shots). The ONLY change is that the CovalX detector position is moved in/out of the flight path. The spectra shown were acquired within minutes (sometimes seconds) of one another. Shown spectra have no smoothing or data processing applied. However, the FlashDetector spectra were recalibrated to show correct masses because of the differences in flight times between the two detectors Instruments Incorporated, Saugus, MA Basic Science Institute, Daejeon, SOUTH KOREA 3CovalX AG, Zürich, SWITZERLAND www.covallx.com [email protected] Results/Spectra Immunoglobulin M 0.6μM UltraFlextreme FlashDetector CovalX HM2 5IgG + + IgM +2 UltraFlextreme Flash Detector CovalX HM2 IgM + Conclusions While the latest FlashDetector technology utilized in the Bruker UltraFlex system provides noticeable improvement over the MCP technology utilized in previous Bruker instruments; there is still a significant difference in detection efficiency when compared to the CovalX High Mass Systems. Approximately twice as large of ion masses are detected under identical conditions when using the CovalX high mass systems. There is also a noticeable increase in total ion intensity measured and signal-to-noise with the CovalX system These detection differences become more noticeable the higher in mass that ions are measured or the more complex the sample signal is. Acknowledgments The authors acknowledge SunMoon Min from SMAnalytical and the researchers at KBSI for coordinating this work. The authors also acknowledge Jan Streller and the rest of the Bruker team which made this installation such a smooth process.
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Figure 2. Comparison between standard detection (red) and HM2
high-mass detection (blue) for 4 proteins (A: Insulin, B: BSA, C: IgG and
D: IgM). Each sample is analyzed from the same spot under ide...