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Titlebook: HPLC of Peptides and Proteins; Methods and Protocol Marie-Isabel Aguilar Book 2004 Humana Press 2004

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https://doi.org/10.1007/978-94-015-2747-7d first published in 1963 (.). During the 1970s, the first automation of peptide synthesis was undertaken using Boc chemistry. In the 1980s, improvements were made in the Boc chemistry automated process and, consequently, the synthesis of more-difficult sequences, as well as longer polypeptides beca
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https://doi.org/10.1007/978-3-319-76956-1volving the processing of liters or hundred liters of material, requires chromatographic principles to be applied within the boundaries imposed by economic, regulatory, and engineering constraints. In fact, the actual chromatographic process used at large scale is dictated equally by these factors a
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https://doi.org/10.1007/978-1-4615-1063-5y be able to tell whether the protein has the expected mass. If you find a deviation from the expected you will, in most cases, be left wondering where (and perhaps what) the difference is. These observations are compounded when using low-resolution techniques like gel filtration or sodium dodecyl s
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HPLC of Peptides and Proteinsmolecules. In particular, HPLC in its various modes has become the central technique in the characterization of peptides and proteins and has, therefore, played a critical role in the rapid advances in the biological and biomedical sciences over the last 10 years.
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Reversed-Phase High-Performance Liquid Chromatographypends on the hydrophobic binding of the solute molecule from the mobile phase to the immobilized hydrophobic ligands attached to the stationary phase, i.e., the sorbent. A schematic diagram showing the binding of a peptide or a protein to a reversed-phase surface is shown in .. The solute mixture is
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