All WAVEsystem products have been designed with user experience in mind. At the same time, they are highly sophisticated bioanalytical instruments requiring skilled user input.
To help you get the most from your product, we have combined the wealth of our internal knowledge and experience in one practical reference manual. Our experts guide you through the main principles underlying the technologies, techniques and applications. We provide information, advice and tips on experimental design and data analysis. A separate troubleshooting section covers the situations and questions encountered most often by our customer support teams.
Whether you read it from cover to cover, refer to it for specific questions, or keep it as a handy reminder of equations and protocols, we hope that this manual will support you in your work and contribute to results that accelerate discovery.
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| Content | Page |
|---|---|
| 1. Welcome | 5 |
| 2. Introduction | 7 |
| 2.1 Introduction to label-free interaction analysis | 8 |
| 2.1.1 Definitions of label-free terminology | 12 |
| 2.1.2 Principles of label-free analysis | 16 |
| 2.2 The Creoptix WAVEsystem | 19 |
| 2.2.1 GCI technology | 19 |
| 2.2.3 Non-clog microfluidics | 21 |
| 2.2.3 GCI vs other label-free biosensor technologies | 24 |
| 2.3 Overview of applications | 26 |
| 2.3.1 Kinetics and affinity analysis | 26 |
| 2.3.2 Molecular screening | 29 |
| 2.3.3 Binding specificity | 31 |
| 2.3.4 Concentration analysis | 32 |
| 3. Experimental design | 34 |
| 3.1 Sensor Surfaces | 35 |
| 3.1.1 Chip type selection | 35 |
| 3.1.2 Chip conditioning | 40 |
| 3.1.3 Immobilization strategies | 41 |
| 3.1.4 Surface regeneration | 51 |
| 3.1.5 Ligand regeneration | 53 |
| 3.2 Ligand immobilization | 56 |
| 3.2.1 Ligand density | 56 |
| 3.2.2 Ligand activity | 59 |
| 3.2.3 Mass transport limitation | 60 |
| 3.2.4 Ligand avidity | 61 |
| 3.2.5 Non-specific binding | 62 |
| 3.3 Buffer | 63 |
| 3.3.1 General considerations | 63 |
| 3.3.2 Buffer composition | 63 |
| 3.3.3 Buffer/sample matching | 67 |
| 3.4 Referencing and correction | 69 |
| 3.4.1 Referencing | 69 |
| 3.4.2 Double referencing | 69 |
| 3.4.3 DMSO correction (solvent correction) | 70 |
| 3.5 Assay format | 75 |
| 3.5.1 Kinetics and affinity analysis | 75 |
| 3.5.2 Molecular screening | 84 |
| 3.5.3 Binding specificity and competition experiments | 85 |
| 3.5.4 Concentration analysis | 87 |
| 3.5.5 Sample recovery for analyte binder identification | 91 |
| 4. Data analysis | 97 |
| 4.1 Data adjustment | 98 |
| 4.1.1 Signal jumps | 99 |
| 4.1.2 Offsets | 99 |
| 4.1.3 DMSO correction (solvent correction) | 100 |
| 4.1.4 Blanks | 101 |
| 4.2 Data evaluation | 102 |
| 4.2.1 Evaluation output and quality | 103 |
| 4.2.2 Settings and advanced menu | 105 |
| 4.2.3 Model selection | 109 |
| 4.2.4 Equilibrium analysis | 116 |
| 4.3 waveRAPID | 117 |
| 4.4. Screen | 119 |
| 4.4.1 Settings | 119 |
| 4.4.2 Plot data series | 119 |
| 4.4.3 Ranking/hits | 120 |
| 4.4.4 Off-rate screens | 120 |
| 5. Troubleshooting | 122 |
| 5.1 Leakage | 123 |
| 5.2 Device state | 123 |
| 5.3 Distorted signa | 124 |
| 5.3.1 Noisy signal | 124 |
| 5.3.2 Unstable/low amplitudes | 125 |
| 5.3.3 Signal spikes/phase losses | 126 |
| 5.4 Ligand immobilization | 127 |
| 5.4.1 Low binding | 127 |
| 5.4.2 Low ligand activity | 128 |
| 5.5 Kinetics | 128 |
| 5.5.1 No saturation/over-stoichiometric signal | 128 |
| 5.5.2 No dissociation signal/ linear association | 129 |
| 5.5.3 waveRAPID | 129 |
| 6. References | 130 |
All WAVEsystem products have been designed with user experience in mind. At the same time, they are highly sophisticated bioanalytical instruments requiring skilled user input.
To help you get the most from your product, we have combined the wealth of our internal knowledge and experience in one practical reference manual. Our experts guide you through the main principles underlying the technologies, techniques and applications. We provide information, advice and tips on experimental design and data analysis. A separate troubleshooting section covers the situations and questions encountered most often by our customer support teams.
Whether you read it from cover to cover, refer to it for specific questions, or keep it as a handy reminder of equations and protocols, we hope that this manual will support you in your work and contribute to results that accelerate discovery.
| Content | Page |
|---|---|
| 1. Welcome | 5 |
| 2. Introduction | 7 |
| 2.1 Introduction to label-free interaction analysis | 8 |
| 2.1.1 Definitions of label-free terminology | 12 |
| 2.1.2 Principles of label-free analysis | 16 |
| 2.2 The Creoptix WAVEsystem | 19 |
| 2.2.1 GCI technology | 19 |
| 2.2.3 Non-clog microfluidics | 21 |
| 2.2.3 GCI vs other label-free biosensor technologies | 24 |
| 2.3 Overview of applications | 26 |
| 2.3.1 Kinetics and affinity analysis | 26 |
| 2.3.2 Molecular screening | 29 |
| 2.3.3 Binding specificity | 31 |
| 2.3.4 Concentration analysis | 32 |
| 3. Experimental design | 34 |
| 3.1 Sensor Surfaces | 35 |
| 3.1.1 Chip type selection | 35 |
| 3.1.2 Chip conditioning | 40 |
| 3.1.3 Immobilization strategies | 41 |
| 3.1.4 Surface regeneration | 51 |
| 3.1.5 Ligand regeneration | 53 |
| 3.2 Ligand immobilization | 56 |
| 3.2.1 Ligand density | 56 |
| 3.2.2 Ligand activity | 59 |
| 3.2.3 Mass transport limitation | 60 |
| 3.2.4 Ligand avidity | 61 |
| 3.2.5 Non-specific binding | 62 |
| 3.3 Buffer | 63 |
| 3.3.1 General considerations | 63 |
| 3.3.2 Buffer composition | 63 |
| 3.3.3 Buffer/sample matching | 67 |
| 3.4 Referencing and correction | 69 |
| 3.4.1 Referencing | 69 |
| 3.4.2 Double referencing | 69 |
| 3.4.3 DMSO correction (solvent correction) | 70 |
| 3.5 Assay format | 75 |
| 3.5.1 Kinetics and affinity analysis | 75 |
| 3.5.2 Molecular screening | 84 |
| 3.5.3 Binding specificity and competition experiments | 85 |
| 3.5.4 Concentration analysis | 87 |
| 3.5.5 Sample recovery for analyte binder identification | 91 |
| 4. Data analysis | 97 |
| 4.1 Data adjustment | 98 |
| 4.1.1 Signal jumps | 99 |
| 4.1.2 Offsets | 99 |
| 4.1.3 DMSO correction (solvent correction) | 100 |
| 4.1.4 Blanks | 101 |
| 4.2 Data evaluation | 102 |
| 4.2.1 Evaluation output and quality | 103 |
| 4.2.2 Settings and advanced menu | 105 |
| 4.2.3 Model selection | 109 |
| 4.2.4 Equilibrium analysis | 116 |
| 4.3 waveRAPID | 117 |
| 4.4. Screen | 119 |
| 4.4.1 Settings | 119 |
| 4.4.2 Plot data series | 119 |
| 4.4.3 Ranking/hits | 120 |
| 4.4.4 Off-rate screens | 120 |
| 5. Troubleshooting | 122 |
| 5.1 Leakage | 123 |
| 5.2 Device state | 123 |
| 5.3 Distorted signa | 124 |
| 5.3.1 Noisy signal | 124 |
| 5.3.2 Unstable/low amplitudes | 125 |
| 5.3.3 Signal spikes/phase losses | 126 |
| 5.4 Ligand immobilization | 127 |
| 5.4.1 Low binding | 127 |
| 5.4.2 Low ligand activity | 128 |
| 5.5 Kinetics | 128 |
| 5.5.1 No saturation/over-stoichiometric signal | 128 |
| 5.5.2 No dissociation signal/ linear association | 129 |
| 5.5.3 waveRAPID | 129 |
| 6. References | 130 |
