Affinity Chromatography



Similar documents
AFFINITY CHROMATOGRAPHY

Affi-Prep Protein A Matrix Instruction Manual

Guide to Reverse Phase SpinColumns Chromatography for Sample Prep

Expression and Purification of Recombinant Protein in bacteria and Yeast. Presented By: Puspa pandey, Mohit sachdeva & Ming yu

Classic Immunoprecipitation

SPE and HPLC. Dr Iva Chianella Lecturer in Analytical Chemistry Cranfield Health +44 (0)

Size Exclusion Chromatography

HiTrap Heparin HP, 1 ml and 5 ml

TECHNICAL BULLETIN. HIS-Select Nickel Affinity Gel. Catalog Number P6611 Storage Temperature 2 8 C

Solid Phase Extraction Products PAGE: 1. Introduction of Solid Phase Extraction (SPE) Why Choose Nano-Micro Tech SPE

Protein purification methods, a practical approach

A Novel Bioconjugation Technology

RESOURCE Q, 1 ml and 6 ml RESOURCE S, 1 ml and 6 ml

Blue Sepharose 6 Fast Flow

Affinity Chromatography

Your partner in immunology

Covalent Conjugation to Cytodiagnostics Carboxylated Gold Nanoparticles Tech Note #105

THE His Tag Antibody, mab, Mouse

Antibody Purification and Labeling

Separation of Amino Acids by Paper Chromatography

Bulk Materials for Preparative and Process Chromatography

6 Characterization of Casein and Bovine Serum Albumin


Non Specific Binding (NSB) in Antigen-Antibody Assays

HiTrap Chelating HP, 1 ml and 5 ml

KMS-Specialist & Customized Biosimilar Service

EZ-Link Maleimide-PEO Solid Phase Biotinylation Kit: spin columns

Choose your optimal tools for protein studies

Disaccharides consist of two monosaccharide monomers covalently linked by a glycosidic bond. They function in sugar transport.

Efficient Multi-Well Protein Purification Strategies

Glutathione Resin. User Manual. User Manual. Cat. Nos , , PT (071414)

biomapping FLAG Epitope System Original & Proven System for Demanding Applications

EZ-Link NHS-Biotin Reagents

Lecture 15: Enzymes & Kinetics Mechanisms

HiPer Ion Exchange Chromatography Teaching Kit

Recombinant Enterokinase Kits

Lab 3 Organic Molecules of Biological Importance

Bio-Gel P Polyacrylamide Gel Instruction Manual

8/20/2012 H C OH H R. Proteins

--not necessarily a protein! (all proteins are polypeptides, but the converse is not true)

Data File. Sephadex G-25 media and pre-packed columns. Introduction. Sephadex G-25 Bead structure. Desalting/buffer exchange and gel filtration

Energy & Enzymes. Life requires energy for maintenance of order, growth, and reproduction. The energy living things use is chemical energy.

TCI Chiral HPLC Column

Application Note. Purifying common light-chain bispecific antibodies using MCSGP. Summary

Effective Blocking Procedures

DP419 RNAsimple Total RNA Kit. RNAprep pure Series. DP501 mircute mirna Isolation Kit. DP438 MagGene Viral DNA / RNA Kit. DP405 TRNzol Reagent

Size Exclusion Chromatography

serum protein and A/ G ratio

INSTRUCTION Probemaker

Optimal Conditions for F(ab ) 2 Antibody Fragment Production from Mouse IgG2a

Chapter 3.2» Custom Monoclonal

Application Note. Separation of three monoclonal antibody variants using MCSGP. Summary

Molecular Cell Biology. Prof. D. Karunagaran. Department of Biotechnology. Indian Institute of Technology Madras

GE Healthcare. Hydrophobic Interaction and Reversed Phase Chromatography. Principles and Methods

ENrich SEC 70 ENrich SEC 650 High-Resolution Size Exclusion Columns Instruction Manual

Chapter 2 Antibodies. Contents. Introduction

Protein Purification Handbook

CHAPTER 2 ANTIGEN/ANTIBODY INTERACTIONS

Method Development for Size-Exclusion Chromatography of Monoclonal Antibodies and Higher Order Aggregates

Enzymes reduce the activation energy

Molecular Biology Techniques: A Classroom Laboratory Manual THIRD EDITION

PCR and Sequencing Reaction Clean-Up Kit (Magnetic Bead System) 50 preps Product #60200

Ch18_PT MULTIPLE CHOICE. Choose the one alternative that best completes the statement or answers the question.

A disaccharide is formed when a dehydration reaction joins two monosaccharides. This covalent bond is called a glycosidic linkage.

Protein immunoblotting

INSTRUCTIONS Edition AC

Genomic DNA Clean & Concentrator Catalog Nos. D4010 & D4011

Name Lab #3: Solubility of Organic Compounds Objectives: Introduction: soluble insoluble partially soluble miscible immiscible

Worksheet Chapter 13: Human biochemistry glossary

1. The diagram below represents a biological process

USP L Phase Listing. Octadecyl silane chemically bonded to porous silica or ceramic micro-particles, 3 to 10 μm in diameter, or a monolithic rod.

Enzyme Activity and Assays

Carbohydrates, proteins and lipids

CHAPTER 1 INTRODUCTION

CUSTOM ANTIBODIES. Fully customised services: rat and murine monoclonals, rat and rabbit polyclonals, antibody characterisation, antigen preparation

Enzymes: Practice Questions #1

A. A peptide with 12 amino acids has the following amino acid composition: 2 Met, 1 Tyr, 1 Trp, 2 Glu, 1 Lys, 1 Arg, 1 Thr, 1 Asn, 1 Ile, 1 Cys

Genomic DNA Extraction Kit INSTRUCTION MANUAL

Size Exclusion Chromatography

Interim Progress Report R&D Project 348. Development of a Field Test Kit for Detection of Blue-Green Algal Toxins

About the Kits...2 Description 2 Components 2. Factor Xa Cleavage...3 Small scale optimization 3 Scale-up 3 Monitoring cleavage 4

Purification of GST-tagged Proteins

About the Kits...2 Description 2 Components 2

Guide to Purification of Polyclonal Antibodies

Methods of Grading S/N Style of grading Percentage Score 1 Attendance, class work and assignment 10 2 Test 20 3 Examination 70 Total 100

The Use of Antibodies in Immunoassays

Rubisco; easy Purification and Immunochemical Determination

Technical Guide for ELISA - Protocols - Troubleshooting

Chemistry 20 Chapters 15 Enzymes

Workshop February 2006

How To Understand The Chemistry Of Organic Molecules

Aspects of industrial purification of peptides using large-scale chromatography. Lars Andersson and Jonas Persson

Chapter 6. Antigen-Antibody Properties 10/3/2012. Antigen-Antibody Interactions: Principles and Applications. Precipitin reactions

Name: Hour: Elements & Macromolecules in Organisms

Marmara Üniversitesi Fen-Edebiyat Fakültesi Kimya Bölümü / Biyokimya Anabilim Dalı PURIFICATION AND CHARACTERIZATION OF PROTEINS

The Thermo Scientific KingFisher Family

50 g 650 L. *Average yields will vary depending upon a number of factors including type of phage, growth conditions used and developmental stage.

IAM Chromatography. HPLC Separation Tools for Membrane Protein Purification and Drug Membrane Permeability Prediction

Chapter 3 Molecules of Cells

Two-Dimensional Gel Electrophoresis (2-DGE)

Transcription:

A successful affinity separation requires a biospecific ligand covalently attached to a chromatographic bed material, the matrix. Properties of affinity matrices are presented in the table below. These properties will differ with the ligand bound. For example, the Toyopearl matrix is stable at ph 2-12, but the specific ligand chemistry may limit the usable range. Toyopearl Epoxy media are used at ph 9-11, 40 C to make a stable secondary amine linkage, but at ph 7-8, 25 C for a stable sulfide linkage. Affinity Matrices Matrix Acrylic Beads PH Range 150 μm cleaning: 0-12 operating: 5-9 Agarose, Beaded 2%: 60-200 μm 4%: 45-165 μm 6%: 45-165 μm Cellulose fibrous tubes, 30-60 μm diam., 6%: 45-165 μm Sepharose 2B: 60-200 μm 4B: 45-165 μm 6B: 45-165 μm Max. Operating Pressure & Flow 0.2 MPa, 100 ml/min (2 x 28 cm column) 4-9 2%: 0.04 MPa, 0.8 ml/min 4%: 0.08 MPa, 1.0 ml/min 6%: 0.20 MPa, 1.2 ml/min (2.5 x 30 cm column) 2-10 0.07 MPa, 2.4 ml/min (2.5 cm column diameter) 4-9 2B: 0.04 MPa, 0.8 ml/min 4B: 0.08 MPa, 1.0 ml/min 6B: 0.20 MPa, 1.2 ml/min (2.5 x 30 cm column) Properties/Limitations Macroporous; stable in organics; hydrophilic, neutral; no shrinking/swelling with changes in ionic strength; mechanically stable; high binding capacity Analytes up to 4 x 10 7 MW; temperature to 40 C; sterilizable (chemical); insoluble in all common solvents; should not be used with oxidizing agents or chaotropic salts Low resolution; pliable material Analytes up to 4 x 10 7 MW; temperature to 40 C; sterilizable (chemical); insoluble in all common solvents; should not be used with oxidizing agents or chaotropic salts Sepharose CL 2B: 60-200 μm 4B: 45-165 μm 6B: 45-165 μm Toyopearl 40-90 μm operating: 2-12 cleaning: 1-13 3-14 CL-2B: 0.05 MPa, 1.2 ml/min CL-4B: 0.12 MPa, 2.2 ml/min CL-6B: 0.20 MPa, 2.5 ml/min (2.5 x 30 cm column) Analytes up to 4 x 10 7 MW; high flow rates; sterilizable (autoclave/chemical); insoluble in all common solvents; can be used in dissociating media, high concentrations of chaotropic salts 0.7 MPa Analytes up to 1 x 10 6 MW; 1000 Å pores; hydrophilic, neutral; compatible with solvents; chemically resistant; volume stable to changes in ph or ionic strength 80 cm H 2 O = 0.8 bar = 11.6 psi = 0.08 MPa. 4 ORDER: 800-325-3010 TECHNICAL SERVICE: 800-325-5832 sigma.com

Affinity Ligands The ligand should exhibit specific and reversible binding affinity for the substance to be purified. In addition, it should have chemically modifiable groups that allow it to be attached to the matrix without destroying its ligand-binding activity. The dissociation constant (K d ) for the ligand binding substance complex should ideally be in the range of 10-4 to 10-8 M in free solution. If no information is available on the strength of the binding complex, use a trial and error approach. It is important to consider the region of the ligand that will be used for attachment to the matrix. If several functional groups are available, the ligand should be coupled via the group least likely to be involved in the specific interaction with the molecule to be isolated. Spacer Arms The active site on a biological molecule is often located deep within the molecule. Adsorbents prepared by coupling small ligands directly to the matrix can exhibit low capacities, due to steric hindrance. To prevent this, a spacer arm can be used between the matrix and ligand, to facilitate effective binding. Alternatively, if the spacer arm is too long, nonspecific effects become pronounced and reduce the selectivity of the separation. Affinity Media Group-specific media have affinity for a group of related compounds, rather than for a single substance, thus enabling the analyst to use the same general ligand to purify several substances (e.g., a class of enzymes). Within the group there is either a structural or functional similarity. For example, heparin-bearing affinity media recognize b-pleated sheet domains. Thus, heparin media are useful for purifying coagulation factors, lipoproteins and lipoprotein lipases, growth factors, and enzymes active in nucleic acid metabolism. Activated media are resins with activated functional groups ready for direct coupling of a protein or other ligand. The cyanogen bromide-activated matrices are typical examples. The reaction of cyanogen bromide with the matrix activates the product to which proteins, nucleic acids, or other biopolymers then can be coupled, under mild conditions, via primary amino or similar nucleophilic groups. Resins with reactive groups employ carbodiimide coupling or reductive amination to achieve covalent bonding. For example, the Toyopearl AF-Amino-650M matrix can be used to couple ligands via their carboxylate groups (peptide bond formation) or aldehyde groups (reductive amination). Aldehyde groups may be present in a carbohydrate or glycoprotein ligand, or can be introduced into the intended ligand by mild periodate oxidation. This reactive matrix is used for coupling either proteins or low molecular weight ligands (e.g., lactose). Our Innovation, Your Research Shaping the Future of Life Science 5

Applications for Affinity Media Affinity Class Activated Amino Acid Avidin & Biotin Carbohydrate Dye Glutathione Hydrophobic Potential Applications Functional spacer; support matrix; eliminates handling of toxic reagents. Serum proteins; proteins; peptides; enzymes; rrna; dsdna. Purification of biotin/avidin & derivatives; biotinylated substances. Biotin derivatives dissociate under nondenaturing conditions. Glycoproteins; lectins; other carbohydrate metabolite proteins. Proper selection can ensure one-step purification. Nonspecific interaction. Mimic biological substances (substrates, cofactors, effectors); proteins. Optimize purification protocol with different dyes. Detoxification enzymes; glutathione S-transferase and fusion proteins; glutathione peroxidase and glyoxalase. Couple ligands containing free carboxyl groups; proteins. Immunochemical Lectin Nucleotide/Coenzyme Nucleic Acid Specialty Removal of antibodies from antisera or serum proteins. Solid phase second antibodies. Soluble glycoproteins; other carbohydrate-containing substances. Dehydrogenases; kinases; transaminases. Reliable adsorbents. mrna; DNA; rrna; other nucleic acids and oligonucleotides. Purification of specific classes or types of proteins, coenzymes, or physiological partners. Toyopearl Resins Group Specific Activated Reactive Large pore diameter; medium pressure. Nucleotide-dependent enzymes; bind histidine and free cysteines of peptides or proteins; purify coagulation factors; lipoproteins; enzymes active in nucleic acid metabolism. Large pore diameter; medium pressure; optimal ph 7-9; highly reactive to amine/ thiol groups. Immobilize protein or low MW ligands. Large pore diameter; medium pressure; ph range 6.9-9 or 4.5-6. Primary amines; carboxylate, aldehyde, or amino groups. 6 ORDER: 800-325-3010 TECHNICAL SERVICE: 800-325-5832 sigma.com

Recommended Reading : Principles & Methods This handbook serves as an introduction to affinity chromatography and a practical guide to the media developed by Pharmacia Biotech. The text covers ligands, spacers, and coupling gels, and describes general experimental methods...23499 Selective! Get what you want out of your affinity chromatography with Sigma Broad range of ligand groups Optimized ligand immobilization for correct orientation and long life Reliable support matrices minimize non-specific binding, maximize capacity To learn more, visit sigma.com/affinitychrom sigma-aldrich.com Our Innovation, Your Research Shaping the Future of Life Science 7

Products for Ligand TSK-GEL Columns ABA-5PW 7.5 cm 7.5 mm I.D., 10 µm particle size Boronate-5PW 7.5 cm 7.5 mm I.D., 10 µm particle size Adsorption Capacity (per ml gel) Typical Uses p-aminobenzamidine 3-4 mg trypsin trypsin, bovine thrombin, urokinase, enterokinase, plasminogen activator m-aminophenylboronic acid 40 µmol sorbitol glycoproteins, nucleases, nucleotides, catecholamines, carbohydrates, transfer RNAs 813067 813066 Chelate-5PW 7.5 cm 7.5 mm I.D., 10 µm particle size iminodiacetic acid ~20 µmol Cu 2+ or Zn 2+ serum proteins, interferon, collagenase, granule protein, plasminogen activator, lactoferrin 808645 Guard Column Kit: Chelate-5PW 1 cm 6.0 mm I.D., 20 µm particle size na na Guard column 808647 Media for Epitope Tag Purification GST Glutathione Agarose FLAG FLAG Immunoprecipitation Kit ANTI-FLAG M1 Agarose Affinity Gel ANTI-FLAG M2 Affinity Gel EZview TM Red ANTI-FLAG M2 Affinity Gel HISTIDINE HIS-Select Cobalt Affinity Gel HIS-Select Nickel Affinity Gel HIS-Select HF Nickel Affinity Gel EZview Red HIS-Select HC Nickel Affinity Gel Monoclonal Anti-polyHistidine Agarose G4510 FLAGIPT1 A4596 A2220 F2426 H8162 P6611 H0537 E3528 A5713 Pre-packed columns HIS-Select Cartridge 1.25 ml Columns HIS-Select Elution Buffer HIS-Select High Flow Cartridge volume 6.4 ml HIS-Select Spin Columns HIS-Select Wash Buffer HIS-Select ilap 5 ml Column 96-well plates HIS-Select Filter Plate HIS-Select High Capacity (HC) Nickel coated plates, clear, polystyrene HIS-Select High Sensitivity (HS) Nickel Coated Plates clear strip-well plate HIS-Select ilap HC Nickel Coated Plate, Clear HA Monoclonal Anti-HA Agarose Anti-HA Immunoprecipitation Kit EZview Red Anti-HA Affinity Gel H8286 H5413 H7163 H7787 H5288 H9913 H0413 S5563 S5688 H9412 A2095 IP0010 E6779 8 ORDER: 800-325-3010 TECHNICAL SERVICE: 800-325-5832 sigma.com

HSV Anti-HSV Agarose Affinity Gel c-myc Anti-c-Myc Agarose Affinity Gel antibody produced in rabbit EZview TM Red Anti-c-Myc Affinity Gel Anti-c-Myc Immunoprecipitation Kit A7220 A7470 E6654 IP0020 PROTEIN A AND G EZview Red Protein A Affinity Gel P6486 Protein A Agarose P2545 Protein A Agarose, 2.5 ml column PA1 Protein A Antibody Purification Kit PURE1A EZview Red Protein G Affinity Gel E3403 Protein G, immobilized on crosslinked 4% agarose 83219 Protein G Immunoprecipitation Kit IP50 Other Affinity Media Heparin, immobilized on Agarose 4B, from porcine intestinal mucosa, BioChemika, for affinity chromatography 51546 Lectin, immobilized on Agarose CL-4B from Triticum vulgaris, BioChemika, for affinity chromatography 61768 Oligo dt-cellulose, BioChemika, for affinity chromatography 75349 ω-aminohexyl Agarose, BioChemika, for affinity chromatography, activated with cyanogen bromide 08055 BIOTIN/STREPTAVIDIN EZview Red Streptavidin Affinity Gel E5529 Biotin Agarose B0519 Streptavidin Agarose from Streptomyces avidinii S1638 Streptavidin, immobilized on Agarose CL-4B 85881 THIOREDOXIN Anti-Thioredoxin Agarose antibody produced in rabbit V5 Anti-V5 Agarose Affinity Gel A2582 A7345 VSV Monoclonal Anti-VSV-Glycoprotein-Agarose A1970 Our Innovation, Your Research Shaping the Future of Life Science 9

2026 © DocPlayer.net Privacy Policy | Terms of Service | Feedback  | Do Not Sell My Personal Information