10420nam 2200469 450 991083016820332120230223131124.03-527-83309-93-527-83308-0(MiAaPQ)EBC7101515(Au-PeEL)EBL7101515(CKB)24949921500041(EXLCZ)992494992150004120230223d2023 uy 0engurcnu||||||||txtrdacontentcrdamediacrrdacarrierCapillary electrophoresis -- mass spectrometry for proteomics and metabolomics principles and applications /edited by Rawi Ramautar and David D. Y. ChenHoboken, New Jersey :John Wiley & Sons,[2023]©20231 online resource (403 pages)Print version: Ramautar, Rawi Capillary Electrophoresis - Mass Spectrometry for Proteomics and Metabolomics Newark : John Wiley & Sons, Incorporated,c2022 9783527349210 Includes bibliographical references and index.Cover -- Title Page -- Copyright -- Contents -- Preface -- Chapter 1 Capillary Electrophoresis-Mass Spectrometry Interfacing: Principles and Recent Developments -- 1.1 Introduction -- 1.2 General Considerations of CE-ESI-MS -- 1.2.1 Electrospray Ionization -- 1.2.2 Electrical Circuit in CE-ESI-MS -- 1.2.3 CE Modes and Conditions in CE-MS -- 1.3 Sheath Liquid Interfaces -- 1.3.1 Coaxial Sheath‐Flow ESI-MS Interface -- 1.3.2 Nanoflow Sheath Liquid ESI-MS Interface -- 1.4 Sheathless Interfaces -- 1.4.1 Porous‐Tip Interface -- 1.4.2 Other Sheathless Interfaces -- 1.5 Other CE-ESI-MS Interfaces -- 1.5.1 Liquid Junction -- 1.5.2 Interface‐Free CE-MS -- 1.6 Microchip Electrophoresis-MS Interfaces -- 1.7 Alternative Ionization Techniques for CE-MS -- 1.7.1 CE and MCE Combined with MALDI-MS -- 1.7.2 CE-ICP-MS -- 1.8 Concluding Remarks and Outlook -- List of Abbreviations -- References -- Chapter 2 Data Analysis Strategies in CE-MS for Metabolomics -- 2.1 Introduction -- 2.2 The Annotation Challenge in CE-MS‐Based Untargeted Metabolomics -- 2.2.1 Peak Picking in CE-MS Metabolomics -- 2.2.2 Alignment Approaches -- 2.2.3 μeff Transformation -- 2.2.3.1 Historical Evolution and Current State -- 2.2.3.2 Quantitative Aspects of the Use of Mobilograms -- 2.2.3.3 Technical Considerations of the μeff Transformation -- 2.2.4 Reproducibility and Exchange of μeff Information Using Libraries -- 2.2.5 Interlaboratory Reproducibility -- 2.2.6 ROMANCE -- 2.2.7 Ion Mobility -- 2.3 Data Pretreatment -- 2.3.1 Area Normalization -- 2.3.2 Analytical Quality Monitoring -- 2.3.3 Data Filtering -- 2.4 Data Treatment -- 2.5 Concluding Remarks -- Acknowledgment -- References -- Chapter 3 Data‐Processing Workflow for Relative Quantification from Label‐Free and Isobaric Labeling‐Based Untargeted Shotgun Proteomics: From Database Search to Differential Expression Analysis.3.1 Introduction -- 3.2 Spectra Acquisition and Database Search -- 3.2.1 Parameters Affecting Sequence Database Search -- 3.2.1.1 Database Selection -- 3.2.1.2 Enzyme Specificity and Missed Cleavages -- 3.2.1.3 Posttranslational Modifications -- 3.2.1.4 Precursor Mass Tolerance -- 3.2.2 Target-Decoy Search Strategy for False Discovery Rate Estimation -- 3.2.3 Database Search Engines -- 3.2.3.1 SEQUEST -- 3.2.3.2 Mascot -- 3.2.3.3 Multiple Search Engines -- 3.2.4 Protein Inference -- 3.3 Relative Protein Quantification -- 3.3.1 Filtering -- 3.3.2 Missing Value Imputation -- 3.3.2.1 Imputation Methods -- 3.3.2.2 Comparative Studies -- 3.3.2.3 Normalization -- 3.3.3 Summarization -- 3.3.4 Differential Expression Analysis -- 3.4 Conclusions -- References -- Chapter 4 Data Processing in Metabolomics Capillary Electrophoresis-Mass Spectrometry -- 4.1 Data Extraction and the Interpretation of the Extracted Data -- 4.2 Data Preprocessing -- 4.2.1 Handling Missing Values -- 4.2.2 Normalization -- 4.2.3 Transformation -- 4.2.4 Scaling -- 4.3 Statistical Analysis -- 4.3.1 Two‐Sample T‐Test -- 4.3.2 Principal Component Analysis (PCA) -- 4.3.3 Partial Least‐Squares Discriminant Analysis (PLS-DA) -- 4.3.4 Support Vector Machine -- 4.3.5 Logistic Regression -- 4.3.6 Random Forest Model -- 4.3.7 Evaluation of Classification Models -- 4.4 Metabolite Identification -- References -- Chapter 5 Utility and Advances of Capillary Electrophoresis-Mass Spectrometry for Metabolomics -- 5.1 Introduction -- 5.2 Technological Developments -- 5.2.1 Improving Sensitivity -- 5.2.2 Increasing Metabolome Coverage -- 5.2.3 Increasing Annotation Capacity -- 5.2.4 Tackling Anionic Profiling -- 5.2.5 Increasing Sample Throughput -- 5.3 Applications -- 5.3.1 Biomedical Samples -- 5.3.2 Microbial Extracts -- 5.3.3 Plants -- 5.4 Concluding Remarks -- Acknowledgment -- Conflict of Interest.References -- Chapter 6 Comprehensive Lipid Profiling by Multisegment Injection-Nonaqueous Capillary Electrophoresis-Mass Spectrometry: Expanding Coverage Beyond Hydrophilic Metabolites -- 6.1 The Early Origins of Lipidomics -- 6.2 Major Instrumental Platforms in Lipidomics: The Role of Separation Science -- 6.3 NACE-MS: An Emerging Separation Platform for Lipidomics? -- 6.4 Multiplexed Separations for Fatty Acids by MSI-NACE-MS -- 6.5 Comprehensive Lipid Profiling Strategies by MSI-NACE-MS -- 6.6 Future Perspectives and Summary -- References -- Chapter 7 Strategies for Identification of Modified Amino Acids with CE-MS in Metabolomics -- 7.1 Introduction -- 7.1.1 Post‐Translational Modifications and Modified Amino Acids -- 7.1.2 Modified Amino Acids as Biomarkers of Pathologies -- 7.2 Methods for the Detection of Modified Amino Acids -- 7.3 Capillary Electrophoresis Coupled to Mass Spectrometry to Analyze Modified Amino Acids -- 7.3.1 Applications of CE-MS for Analysis of Modified Amino Acids -- 7.4 Recent Developments to Enhance and Facilitate the Annotation Process in CE-MS -- Acknowledgments -- References -- Chapter 8 CE-MS Approaches for Single‐Cell Metabolomics -- 8.1 Introduction -- 8.2 Techniques for Single‐Cell Metabolome Analysis -- 8.2.1 Highly Sensitive CE-MS Interfacing -- 8.2.2 Online Sample Preconcentration Techniques -- 8.2.3 Isolation of Single Cells -- 8.3 Application to Single‐Cell Metabolome Analysis -- 8.3.1 Metabolome Analysis of Large Single Cells with Highly Sensitive Interface -- 8.3.2 Single‐Cell Metabolome Analysis with Highly Sensitive Interface and OSP Method -- 8.3.3 Single‐Cell Metabolome Analysis by Online Sampling and Highly Sensitive Interface -- 8.4 Conclusions -- References -- Chapter 9 CE-MS Approaches for Peptidomics -- 9.1 Introduction -- 9.2 Sample Preparation -- 9.3 CE-MS -- 9.3.1 Basic Characterization.9.3.2 Peptide Identification -- 9.3.3 Peptide Quantitation -- 9.4 Applications -- 9.4.1 Search, Identification, and Determination of Biomarkers -- 9.4.2 Food Peptidomics -- 9.4.3 Other Applications -- 9.5 Conclusions -- Acknowledgments -- List of Abbreviations -- References -- Chapter 10 Capillary Zone Electrophoresis-Mass Spectrometry for Top‐Down Proteomics: Technological Development and Biological Applications -- 10.1 Introduction -- 10.2 Technological Development -- 10.2.1 CE-MS Interface -- 10.2.2 Capillary Coating -- 10.2.3 Sample Loading Capacity and Separation Window -- 10.2.4 Coupling Novel Gas‐Phase Fragmentation Techniques to CZE-MS/MS for TDP -- 10.2.5 Electrophoretic Mobility Prediction of Proteoforms -- 10.3 Applications of CZE-MS‐Based TDP -- 10.3.1 Delineation of Proteoforms of Complex Proteomes, Disease Biomarkers, and Biopharmaceuticals -- 10.3.2 CZE-MS for Native TDP -- 10.4 Conclusions and Perspectives -- Acknowledgments -- References -- Chapter 11 CE-MS Methods for the Characterization of Monoclonal Antibodies -- 11.1 Introduction -- 11.2 mAb Characterization Approaches -- 11.3 Applications -- 11.3.1 Primary Structure Characterization of Monoclonal Antibodies -- 11.3.1.1 Analytical Workflow -- 11.3.1.2 Amino Acid Sequence Characterization Using CE-MS(/MS) -- 11.3.1.3 PTMs Characterization and Relative Quantification Using CE-MS(/MS) -- 11.3.1.4 Glycosylation Determination Using CE-MS(/MS) -- 11.3.2 Middle‐Up/Middle‐Down Analysis -- 11.3.2.1 Analytical Workflow -- 11.3.2.2 mAb Analysis Using Middle‐Up Strategy -- 11.3.2.3 mAb Analysis Using Middle-Down Strategy -- 11.3.3 Intact Analysis -- 11.3.3.1 Analytical Workflow -- 11.3.3.2 mAb Analysis in Denaturing Conditions Using CE-MS -- 11.3.3.3 mAb Analysis in Native Conditions Using CE-MS -- 11.3.4 Automation: Future of CE-MS for mAb Analysis -- 11.4 Conclusion -- References.Chapter 12 CE and CE-MS Approaches for Glycan Analysis -- 12.1 The Importance of Glycosylation -- 12.2 Capillary Electrophoresis in Analytical Glycomics -- 12.2.1 Sample Preparation for CE‐Based Glycan Analysis -- 12.2.2 Analysis of Oligosaccharides from Biological Samples -- 12.2.3 Structural Elucidation of Carbohydrates: The GU Value Approach -- 12.2.4 LIF Sensitivity and Quantification -- 12.3 CE-MS of Oligosaccharides -- 12.3.1 Major Parameters to Set the ESI for CE-MS of Derivatized Oligosaccharides -- 12.3.2 CE-MS for Quantitative Carbohydrate Analysis -- 12.3.3 CE-MS for Glycomic Studies -- 12.4 Conclusions and Future Prospective -- Acknowledgment -- References -- Chapter 13 CE-MS Approaches for Glyco(proteo)mic Analysis -- 13.1 Introduction -- 13.1.1 N‐Linked Glycosylation -- 13.1.2 O‐Linked Glycosylation -- 13.1.3 Glycosylation Workflows -- 13.1.4 Analytical Approaches -- 13.1.5 CE-MS Interfaces -- 13.2 Glycan Analysis by CE-MS -- 13.2.1 Glycan Derivatization Strategies -- 13.3 Glycopeptide Analysis -- 13.3.1 Sample Treatment -- 13.3.2 Separation Conditions -- 13.3.3 Applications -- 13.4 Protein Analysis -- 13.4.1 Sample Treatment -- 13.4.2 Separation Conditions -- 13.4.3 Applications -- 13.5 Conclusions and Outlook -- Acknowledgments -- List of Abbreviations -- References -- Index -- EULA.Capillary electrophoresisCapillary electrophoresis.541.372Ramautar RawiChen David D. Y.MiAaPQMiAaPQMiAaPQBOOK9910830168203321Capillary electrophoresis -- mass spectrometry for proteomics and metabolomics3939480UNINA03116nam 2200685Ia 450 991081353230332120200520144314.01-118-04534-31-119-19874-71-281-23749-397866112374930-470-25923-X(CKB)1000000000412353(EBL)333799(OCoLC)608622527(SSID)ssj0000226914(PQKBManifestationID)11184532(PQKBTitleCode)TC0000226914(PQKBWorkID)10260248(PQKB)11268108(MiAaPQ)EBC333799(Au-PeEL)EBL333799(CaPaEBR)ebr10226875(CaONFJC)MIL123749(OCoLC)164803375(FINmELB)ELB177449(EXLCZ)99100000000041235320070813d2008 uy 0engur|n|---|||||txtccrPricing with confidence 10 ways to stop leaving money on the table /Reed K. Holden, Mark R. Burton1st ed.Hoboken, NJ Wileyc20081 online resource (242 p.)Description based upon print version of record.0-470-19757-9 Includes bibliographical references and index.PRICING WITH CONFIDENCE: 10 WAYS TO STOP LEAVING MONEY ON THE TABLE; CONTENTS; ACKNOWLEDGMENTS; INTRODUCTION: WHY PRICING IS SO HARD AND WHY MOST COMPANIES MESS IT UP; Rule One: Replace the Discounting Habit with a Little Arrogance; Rule Two: Understand the Value You Offer to Your Customer; Rule Three: Apply One of Three Simple Pricing Strategies; Rule Four: Play Better Poker with Customers; Rule Five: Price to Increase Profits; Rule Six: Add New Products and Services that Give You Negotiating Flexibility and Growth; Rule Seven: Force Your Competitor to React to Your PricingRule Eight: Build Your Selling BackboneRule Nine: Take Simple Steps to Move from Cost-Plus to Value-Based Pricing; Rule Ten: Price with Confidence: Remember Who You Are; INDEXBad pricing is a great way to destroy your company's value, revenue, and profits. 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