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List of protocols | p. xiii |
Abbreviations | p. xvii |
Principles of enzyme assay and kinetic studies | p. 1 |
Introduction | p. 1 |
Behaviour of assays | p. 1 |
Reaction progress curves | p. 1 |
Initial rate measurements | p. 5 |
Integrated rate equations | p. 6 |
Bursts and lags in progress curves | p. 7 |
Blank rates | p. 11 |
The effects of enzyme concentration | p. 15 |
Direct proportionality | p. 15 |
Upward curvature | p. 17 |
Downward curvature | p. 18 |
Expression of enzyme activity | p. 18 |
Units and specific activity | p. 19 |
The katal | p. 19 |
Stoichiometry | p. 19 |
Conditions for activity measurements | p. 20 |
The effects of substrate concentration | p. 20 |
The Michaelis-Menten relationship | p. 20 |
Failure to obey the Michaelis-Menten equation | p. 21 |
Experimental approaches | p. 29 |
Type of assay | p. 29 |
Choice of assay method | p. 38 |
The effects of pH | p. 39 |
Practical considerations | p. 40 |
Conclusions | p. 44 |
References | p. 44 |
Photometric assays | p. 49 |
Introduction | p. 49 |
Absorption | p. 49 |
Terminology | p. 49 |
Absorbance | p. 50 |
Limitations and sources of error | p. 52 |
Absorbance range | p. 55 |
Measurement of low rates of absorbance change | p. 55 |
Use of absorbance coefficient | p. 56 |
Continuous assays | p. 58 |
Discontinuous assays | p. 63 |
Examples of enzymes assayed by absorbance change | p. 64 |
Turbidimetry | p. 70 |
Fluorescence | p. 71 |
The fluorescence spectrometer | p. 72 |
Quantitation of fluorescence | p. 72 |
Causes of non-linearity - the inner filter effect | p. 73 |
Examples of fluorimetric enzyme assays | p. 73 |
References | p. 77 |
Radiometric assays | p. 79 |
Introduction | p. 79 |
Techniques | p. 80 |
Ion-exchange methods | p. 80 |
Precipitation of macromolecules | p. 81 |
Solvent extraction methods | p. 81 |
Paper and thin-layer chromatographic (TLC) methods | p. 81 |
Electrophoretic methods | p. 81 |
Scintillation Proximity Assay (SPA) | p. 82 |
Experimental design | p. 98 |
Microplate technology | p. 99 |
Measurement of radioactivity | p. 100 |
Automation of assays | p. 100 |
Acknowledgements | p. 100 |
References | p. 100 |
High performance liquid chromatographic assays | p. 103 |
Introduction | p. 103 |
Theory of HPLC | p. 103 |
Introduction | p. 103 |
Chromatographic parameters | p. 104 |
Retention mechanism | p. 106 |
Characteristics of silica | p. 106 |
Polymeric packings | p. 107 |
Reverse phase chromatography | p. 108 |
Influence of composition of mobile phase | p. 111 |
Effect of pH and salts | p. 112 |
Influence of temperature | p. 112 |
Ion-pair chromatography | p. 113 |
Ion-exchange resins | p. 114 |
Size-exclusion chromatography | p. 116 |
Instrumentation | p. 117 |
Essential components of an HPLC system | p. 117 |
Pumps | p. 117 |
Biocompatibility | p. 118 |
Sample injection | p. 118 |
Detectors | p. 119 |
UV/visible detectors | p. 119 |
Fluorescent detectors | p. 120 |
Refractive-index (RI) detectors | p. 121 |
Electrochemical detectors | p. 122 |
Radioactivity monitors | p. 122 |
Practical considerations | p. 123 |
Selection of a chromatographic mode | p. 123 |
Solvent selection | p. 123 |
De-gassing and filtration of solvents | p. 124 |
Sample preparation | p. 124 |
Column packing | p. 124 |
Column protection | p. 125 |
Tubing | p. 125 |
Application of HPLC to enzymatic analysis | p. 125 |
Hydrolases | p. 125 |
Isomerases | p. 127 |
Lyases | p. 130 |
Ligases | p. 133 |
Oxidoreductases | p. 136 |
Transferases | p. 136 |
References | p. 137 |
Electrochemical assays: the oxygen electrode | p. 141 |
Introduction | p. 141 |
Theory and principles | p. 141 |
Current/voltage relationships | p. 142 |
Sensitivity | p. 142 |
Calibration | p. 142 |
Electrode systems | p. 144 |
Polarographic assays | p. 145 |
Tissue/organelle respiration studies | p. 145 |
Specific enzyme studies | p. 146 |
References | p. 148 |
Electrochemical assays: the nitric oxide electrode | p. 149 |
Introduction | p. 149 |
Principles of detection | p. 149 |
Principles of selectivity and sensitivity | p. 149 |
Environmental influences | p. 150 |
Temperature | p. 150 |
Electrical interference | p. 150 |
Membrane integrity and maintenance | p. 151 |
Calibration | p. 151 |
Calibration for liquid measurements | p. 151 |
Calibration for gas-phase measurements | p. 153 |
NO and cellular respiration studies | p. 153 |
References | p. 155 |
Electrochemical assays: the pH-stat | p. 157 |
Introduction | p. 157 |
The basis of pH-stat methodology | p. 157 |
Principle and general approach | p. 157 |
pH-stat components and their functions | p. 158 |
Some limitations and sources of error | p. 159 |
Commercial and custom-made pH-stat assemblies | p. 159 |
The range of equipment | p. 159 |
Some pH-stat systems described in the literature | p. 159 |
General pH-stat procedure and specific protocols for some individual enzymes | p. 162 |
Procedures | p. 162 |
A systematic error in pH-stat assays of enzymes in haemolysates | p. 168 |
Concluding comment | p. 168 |
References | p. 168 |
Enzyme assays after gel electrophoresis | p. 171 |
Introduction | p. 171 |
Preparation of enzyme extracts | p. 171 |
Extraction of microorganisms | p. 171 |
Animal soft tissues | p. 172 |
Mammalian blood | p. 173 |
Insects | p. 173 |
Plant tissues | p. 173 |
Principles of enzyme visualization | p. 175 |
Methods to visualize oxidative enzymes | p. 175 |
Methods to visualize transferases | p. 177 |
Methods to visualize hydrolases | p. 178 |
Methods to visualize lyases, isomerases and ligases | p. 180 |
A compliation of protocols to visualize enzymes following electrophoretic separation | p. 180 |
Staining protocols | p. 184 |
Buffer systems for electrophoresis | p. 201 |
References | p. 206 |
Techniques for enzyme extraction | p. 209 |
Introduction: scope of the chapter | p. 209 |
Disruption of tissues and cells | p. 210 |
Choice of tissue | p. 210 |
Disruption of tissue and separation of cells | p. 211 |
Disruption of cells | p. 212 |
Protection of enzyme activity | p. 215 |
Control of pH | p. 215 |
Control of temperature | p. 215 |
Control of proteolysis | p. 216 |
Protection of thiol groups | p. 217 |
Protection against heavy metals | p. 217 |
Control of mechanical stress | p. 218 |
Effects of dilution | p. 218 |
Assays of enzymes in unfractionated cell-extracts | p. 219 |
The presence of endogenous inhibitors | p. 219 |
Interference from other reactions | p. 219 |
Removal of substrate | p. 219 |
Turbidity of extract | p. 220 |
Concluding remarks | p. 220 |
References | p. 220 |
Buffers and control of pH | p. 221 |
The determination of protein | p. 223 |
References for Appendices | p. 224 |
Determination of active site concentration | p. 225 |
Introduction | p. 225 |
Areas of application | p. 225 |
Categories of titration methods | p. 226 |
Activity bursts | p. 226 |
Inhibitor titration | p. 228 |
Special techniques | p. 230 |
References | p. 233 |
High throughput screening--considerations for enzyme assays | p. 235 |
Introduction | p. 235 |
The drug discovery process | p. 235 |
A historical perspective | p. 235 |
A model of drug discovery | p. 236 |
High throughput screening | p. 237 |
Compounds for screening | p. 239 |
Considerations for high throughput assays | p. 240 |
Enzymatic considerations | p. 245 |
Assay formats for enzymatic HTS | p. 246 |
Automation | p. 246 |
Developments | p. 247 |
Higher density plates | p. 247 |
References | p. 247 |
Statistical analysis of enzyme kinetic data | p. 249 |
Introduction | p. 249 |
Derivation of relationships | p. 250 |
Defining objectives | p. 250 |
Basic assumptions of least squares | p. 251 |
Fitting the Michaelis-Menten equation | p. 252 |
Equations with more than two parameters | p. 258 |
Detecting lack of fit | p. 258 |
Estimating pure error | p. 260 |
Distribution-free methods | p. 262 |
Residual plots | p. 264 |
A note about rounding | p. 267 |
References | p. 268 |
List of suppliers | p. 269 |
Enzyme index | p. 273 |
General index | p. 277 |
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