BioHPLC Column Selection Guide Cover - Agilent Technologies

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ion-exchange Chromatography 4 www.agilent.com/chem/biohplc iOn-eXCHanGe CHROMaTOGRaPHY Purify proteins and other charged molecules Ion-exchange chromatography (IEX) is a highly sensitive technique that allows you to separate ions and polar molecules based on their charge. Like SEC, IEX can be used to separate proteins in their native state. Applying IEX to charge variant analysis During production and purification, antibodies can exhibit changes in charge heterogeneity as a result of amino acid substitutions, glycosylation, phosphorylation, and other post-translational or chemical modifications. Because these changes can impact stability and activity – or cause immunologically adverse reactions – the analysis of charge heterogeneity in monoclonal antibody (MAb) preparations is critical to biopharmaceuticals. In protein analysis, charge variations at a given pH indicate a change in the primary molecular structure – resulting in additional forms of the protein in question. These are called isoforms (or charge variants), and can be resolved by IEX chromatography. IEX is also useful as a preparative technique. The pages that follow describe Agilent’s family of weak and strong ion-exchangers – both anionic and cationic. • Agilent non-porous Bio IEX columns are designed for high-resolution, high-efficiency, and high-recovery separations. • Agilent Bio MAb columns are optimized for separating charge isoforms of monoclonal antibodies. • Agilent porous IEX columns (PL-SAX and PL-SCX) are chemically stable, and are available in two pore sizes – allowing you to separate peptides, oligonucleotides, and very large proteins. • Bio-Monolith IEX columns are uniquely suited to separating antibodies, viruses, and DNA.
Ion-Exchange Column Selection Application Agilent Columns Notes ion-exchange Chromatography Monoclonal antibodies Agilent Bio MAb Thorough characterization of monoclonal antibodies includes the identification and monitoring of acidic and basic isoforms. Agilent Bio MAb HPLC columns feature a unique resin specifically designed for high-resolution charge-based separations of monoclonal antibodies. Peptides and proteins Agilent Bio IEX Agilent Bio Ion-Exchange columns are packed with polymeric, nonporous, ion-exchange particles. Bio IEX columns are designed for high resolution, high recovery and highly efficient separations. Proteins, peptides and deprotected synthetic oligonucleotides PL-SAX The strong anion-exchange functionality, covalently linked to a fully porous chemically � 1000Å � 4000Å stable polymer, extends the operating pH range. In addition, the anion-exchange capacity is independent of pH. For synthetic oligonucleotides, separations using denaturing conditions of temperature, organic solvent, and high pH are all possible. The 5 µm media delivers separations at high resolution with the 30 µm media used for medium pressure liquid chromatography. Globular proteins and peptides PL-SAX 1000Å Very large biomolecules/high speed PL-SAX 4000Å Small peptides to large proteins PL-SCX PL-SCX is a macroporous PS/DVB matrix with a very hydrophilic coating and strong � 1000Å � 4000Å cation-exchange functionality. This process is controlled to provide the optimum density of strong cation-exchange moieties for the analysis, separation and purification of a wide range of biomolecules. The 5 µm media delivers separations at higher Globular proteins PL-SCX 1000Å resolution with the 30 µm media used for medium pressure liquid chromatography. Very large biomolecules/high speed PL-SCX 4000Å Antibodies (IgG, IgM), Bio-Monolith Strong cation-exchange, strong and weak anion-exchange, and Protein A phases. plasmid DNA, viruses, phages and other macro biomolecules � Bio-Monolith QA � Bio-Monolith DEAE � Bio-Monolith SO3 � Bio-Monolith Protein A Bio-Monolith HPLC columns are compatible with preparative LC systems, including Agilent 1100 and 1200 HPLC systems. Viruses, DNA, large proteins Bio-Monolith QA Plasmid DNS, bacteriophages Bio-Monolith DEAE Proteins, antibodies Bio-Monolith SO3 UHPLC/HPLC 4
Page 1 and 2: Agilent BioHPLC Column Selection Gu
Page 3 and 4: BIOCOLUMN SELECTION GUIDELINES From
Page 5 and 6: Column Selection Flow Chart Biocolu
Page 7 and 8: Protein Column Selection Guide Appl
Page 9 and 10: Separation of charge variants of hu
Page 11 and 12: Increased resolution for peptide ma
Page 13 and 14: Preparative scale purification of L
Page 15 and 16: DNA and RNA Oligonucleotide Column
Page 17 and 18: Broad Distribution Biomolecules Car
Page 19 and 20: ReveRseD-PHase HPLC Confidently per
Page 21 and 22: Sterically Protected 300StableBond
Page 23 and 24: Improved reproducibility of monoclo
Page 25 and 26: Short-chain ZORBAX 300SB-C3 is stab
Page 27 and 28: ZORBAX 300Å StableBond Hardware De
Page 29 and 30: LC/MS analysis of angiotensin on Ex
Page 31 and 32: Tips & Tools ZORBAX 300Å Extend-C1
Page 33 and 34: Poroshell 300 columns separate prot
Page 35 and 36: Monoclonal IgG1 chains: Separation
Page 37 and 38: Poroshell 120 • 120Å pore size f
Page 39 and 40: 0 µm 0 µm 0 µm A B C Scanning el
Page 41 and 42: Exploiting chemical stability - TFA
Page 43 and 44: Temperature as a tool to enhance ma
Page 45 and 46: ZORBaX amino acid analysis (aaa) Co
Page 47: High resolution of 24 amino acids u
Page 51 and 52: Consistent ion-exchange MAb separat
Page 53 and 54: Column Specifications Tips & Tools
Page 55 and 56: Weak cation-exchange chromatography
Page 57 and 58: PL-SAX Strong Anion-Exchange Column
Page 59 and 60: Analysis of representative whey pro
Page 61 and 62: Standard protein separation Column:
Page 63 and 64: Agilent Bio-Monolith HPLC Column Se
Page 65 and 66: Baseline expansion of a separation
Page 67 and 68: size exclusion Chromatography (seC)
Page 69 and 70: Column Specifications Agilent Bio S
Page 71 and 72: Comparison of Agilent Bio SEC-3 and
Page 73 and 74: Column Length size exclusion Chroma
Page 75 and 76: Column Specifications Agilent Bio S
Page 77 and 78: Calibration curves - Bio SEC-5 Colu
Page 79 and 80: ProSEC 300S • Mechanically robust
Page 81 and 82: Overlay of UV and light scattering
Page 83 and 84: Retention volume versus log (MW) fo
Page 85 and 86: Agilent PL aquagel-OH SEC Columns f
Page 87 and 88: Heparin Column: 2 x PL aquagel-OH 3
Page 89 and 90: Polyethylene Glycol/Oxide standards
Page 91 and 92: aFFiniTY CHROMaTOGRaPHY Agilent Bio
Page 93 and 94: Rapid human polyclonal IgG quantifi
Page 95 and 96: Multiple Affinity Removal System af
Page 97 and 98: Illustration of high abundance prot
Page 99 and 100:
mRP-C18 High-Recovery Protein Colum
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MeTHOD DeveLOPMenT ZORBAX Column Me
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Reversed-Phase LC/MS Methods Method
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Method Development Ionic Strength:
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Method Development After the initia
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Tips & Tools Agilent offers a varie
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Human serum: Low abundance protein
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2-D LC/MS Analyses Using ZORBAX Cap
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ZORBAX Bio-SCX Series II Capillary
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ZORBAX HPLC Capillary Columns (glas
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Microbore HPLC for sensitive peptid
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BioPharmaceutical Lifecycle Reverse
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ZORBAX 300Å StableBond ZORBAX Prep
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PLRP-S Prep to Process Application
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Prep to Process PLRP-S Size (mm) Pa
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PL-SAX AND PL-SCX FOR PREP TO PROCE
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Prep to Process PL-SAX and PL-SCX D
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Crude peptide screen Column: VariTi
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CARTRIDGE COLUMN SYSTEMS Cartridge
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USP DESIGNATIONS - BIOHPLC COLUMNS
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BioHPLC Columns Literature Title Ag
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BioHPLC Columns Literature Title An
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BioHPLC Columns Literature Title Co
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BIOPHARM DEFINITIONS A active start
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dimer A polymer made up of two iden
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K-L ligase An enzyme that causes mo
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S secondary structure In proteins,
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Poroshell 300 Citations Matilainen,
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Agilent 1260 Infinity Bio-inert Qua
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