The applications and interest in thermal analysis and calorimetry have grown enormously during the last half of the 20th century. These techniques have become indispensable in the study of processes such as catalysis, hazards evaluation etc., and in measuring important physical properties quickly, conveniently and with markedly improved accuracy. Consequently, thermal analysis and calorimetry have grown in stature and more scientists and engineers have become at least part-time, practitioners. People new to the field therefore need a source of information describing the basic principles and current state of the art. The last volume of this 4 volume handbook, devoted to many aspects of biological thermal analysis and calorimetry, completes a comprehensive review of this important area. All chapters have been prepared by recognized experts in their respective fields. The approach taken is "e;how and what to do and when to do it"e;. The complete work is a valuable addition to the already existing literature.
Front Cover 1
Handbook of Thermal Analysis and Calorimetry: From Macromolecules to Man 2
Copyright Page 5
Contents 10
Foreward 6
Preface 8
Contributors 27
CHAPTER 1. ENERGETICS THAT CONTROL THE STABILITY AND DYNAMICS OF SECONDARY AND TERTIARY STRUCTURE OF NUCLEIC ACIDS 30
1. Introduction: Current Advances in the Studies of DNA and RNA Structures 30
2. The DNA World 31
3. The RNA World 63
References 83
CHAPTER 2. THEORY AND PRACTICE OF DSC MEASUREMENTS ON PROTEINS 92
1. Introduction 92
2. The DSC-experiment 92
3. Thermodynamic analysis of heat capacity curves 94
4. Predicting the Cp value of the denatured state on the basis of model compounds 105
5. Analysis of heat capacity curves by statistical physics 110
6. Treatment of irreversible transitions 123
7. Response of the calorimeter 127
8. DSC calorimeter types, practical hints 129
9. Fit Macros 130
References 135
CHAPTER 3. LIPID MODEL MEMBRANES AND BIOMEMBRANES 138
1. Introduction 138
2. Differential scanning calorimetry of membranes 147
3. Isothermal titration calorimetry (ITC) 175
4. Conclusions 196
References 197
CHAPTER 4. COMBUSTION CALORIMETRY 204
1. Introduction 204
2. Sample preparation 211
3. Combustion of microbial samples 215
4. Combustion of plant material 217
5. Combustion of animal material 222
6. Combustion of ecological material 230
7. Conclusions 240
References 241
CHAPTER 5. THE THERMODYNAMICS OF MICROBIAL GROWTH 248
1. Introduction 248
2. Material growth process systems 249
3. The thermodynamics of growth process systems 267
References 293
CHAPTER 6. QUANTITATIVE CALORIMETRY AND BIOCHEMICAL ENGINEERING 296
1. Introduction: Applications of calorimetry in biochemical engineering 296
2. Heat flow rate measurement 298
3. Mole and enthalpy balances in open systems 307
4. Elemental composition 316
5. Enthalpy of combustion of biomass 333
6. Detection and correction of measurement errors 335
7. Energetics of microorganisms 348
8. Calorimetric investigation of multiple limited growth 362
9. Monitoring of aerobic bioprocesses by calorimetry 368
10. Monitoring of anaerobic bioprocesses by calorimetry 373
11. Control of bioprocesses based on calorimetric measurements 376
12. Conclusions 390
References 391
CHAPTER 7. CALORIMETRY OF MICROBLAL PROCESSES 396
1. Background 396
2. The origin of heat production in metabolism 400
3. Future areas of applied calorimetry 407
4. Conclusions 428
References 429
CHAPTER 8. CALORIMETRY OF SMALL ANIMALS 434
1. Introduction 434
2. Direct and indirect calorimetry 439
3. Additional equipment 444
4. Amphibia and reptilia 452
5. Insects 455
6. Protozoa 473
7. Aquatic animals 474
8. Ecology 483
9. Conclusions and perspectives 486
References 488
CHAPTER 9. CALORIMETRIC APPROACHES TO ANIMAL PHYSIOLOGY AND BIOENERGETICS 498
1. Introduction 498
2. Metabolic status and the CR ratio 499
3. Heat flux and oxygen limitation 505
4. Developmental physiology 514
5. Quiescence and diapause 519
6. Nitrate respiration in a clam-bacterium symbiosis 529
7. Conclusions and future directions 532
References 533
CHAPTER 10. WHOLE BODY CALORIMETRY 540
1. Introduction 540
2. Basics 542
3. Methods and equipment 543
4. Whole body calorimetry in biological and nutritional research 568
5. Conclusions 582
References 582
CHAPTER 11. MICROCALORIMETRIC STUDIES OF ANIMAL TISSUES AND THEIR ISOLATED CELLS 586
1. Introduction 586
2. Thermodynamics 587
3. Reasons for systematic errors in calorimetry 591
4. Tissues/Organs 606
5. Cells 620
6. Conclusions 678
References 679
CHAPTER 12. CALORIMETRIC STUDIES IN MEDICINE 686
1. Hematology 686
2. Malignancy 695
3. Immunology 700
4. Endocrinology 705
5. Cardiovascular system 710
6. Nutritional and metabolic disorders 719
7. Kidney 727
References 734
CHAPTER 13. CALORIMERIC METHODS FOR ANALYSIS OF PLANT METABOISM 740
1. Background and general methods 740
2. Plant growth model 762
3. Applications 768
References 786
CHAPTER 14. WOOD 794
1. Introduction 794
2. Characteristics of Wood 795
3. Investigations on wood 796
4. Pyrolysis of wood 797
5. Pyrolysis of wood components 799
6. Wood and fire retardants 802
7. Wood and synthetic polymers 805
8. Wood and water 806
9. Energy content of wood 808
10. Aging and fossilization of wood 815
11. Wood for musical instruments 817
12. Wood and paper 820
13. Wood and wasp nests 826
14. Microbial degradation of wood 827
15. Other observations on wood 831
16. Conclusion 832
References 832
CHAPTER 15. DYNAMIC MECHANICAL ANALYSIS OF ELASTOMERS 840
1. Introduction 840
2. Temperature dependence of relaxation 843
3. Compounding variables 850
References 855
CHAPTER 16. THERMAL ANALYSES IN FOODS AND FOOD PROCESSES 858
1. Introduction 858
2. Phase diagrams 865
3. Cereal Products 868
4. Proteins 892
Appendix 925
References 940
CHAPTER 17. THERMAL ANALYSIS AND CALORIMETRY OF PHARMACEUTICALS 952
1. Introduction 952
2. Characterisation of pharmaceutical solids 953
3. Chemical stability studies 980
4. Miscellaneous uses 1005
References 1038
INDEX 1046
Theory and Practice of DSC Measurements on Proteins
Jörg Rösgen; Hans-Jürgen Hinz Institut für Physikalische Chemie, Westfälische Wilhelms Universität Münster, Schloβplatz 7, 48149 Münster, Germany
1 INTRODUCTION
Proteins are fascinating biological and physical objects. The investigation of protein energetics is not only important for the understanding of their biological function, such studies have also an intrinsic heuristic value for the rationalisation of some unique physical properties of proteins that result from the small size of these macromolecules compared to the magnitude of standard classical thermodynamic systems [1]. The understanding of the physical properties of proteins will also enhance the understanding of their biological reactions.
Experimental access to the energetic properties of proteins can be obtained by several methods. However, none of these methods provide such a direct and powerful approach as differential scanning calorimetry. DSC monitors the response function “heat capacity” which is directly related to the partition function of the system. Knowledge of the partition function is sufficient to derive all the thermodynamic information on the system.
2 THE DSC-EXPERIMENT
2.1 Sample preparation
An important starting point for a successful DSC experiment is the careful preparation of all solutions. Generally the buffer should be filtered and degassed. The sample solution should be essentially free of oxygen, especially if there are free cysteines in the protein [2]. If ligands are involved, their concentrations have to be adjusted with great care. This is also true of H+ ions as ligands. For example, in some cases pH-shifts of a few tenth of a pH unit can result in remarkable shifts in the unfolding temperature of a protein [3].
The protein must be dialysed exhaustively against buffer before the measurement. Typical protein concentrations that can be measured accurately by present day DSC instrumentation are in the range of 0.1 mg/ml to 10 mg/ml. High concentrations yield a favourable signal to noise ratio, but they may favour unspecific irreversible aggregation of the samples.
2.2 Measurement and data treatment
DSC monitors the energy needed to raise the temperature of the sample. Heating rates between 0.1 and 2 K/min are routinely employed with protein solutions. The temperature scans must be done with both the sample and the equilibrium dialysis buffer solution. The difference in heat capacity between these solutions – the so-called apparent heat capacity ΔCp,app – is the basis for all Cp calculations.
This difference originates from the replacement of buffer solution by proteins. The corresponding equation is:
Cp,app=cp,buffer·mbuffer−cp,protein·mprotein,
(1)
where mbuffer and 'mprotein are, respectively, the mass of the replaced buffer and the protein. Introducing the specific volume v = V/m and solving for the heat capacity of the protein one obtains the equation
p,protein=Cp,buffer·vproteinvbuffer−ΔCp,appmprotein.
(2)
At low buffer concentration the heat capacity of the buffer is not very different from the heat capacity of water. Therefore often the heat capacity of water at room temperature (1 cal/gK = 4.184 J/gK) is used as an approximate value for the specific: heat capacity of the buffer cp,buffer. However, if accurate data are needed, a third measurement of water against buffer must be performed, which yields the difference in heat capacity between buffer and water. Since the heat capacity of water is known accurately and can be expressed by the following polynomial equation based on the data of Stimson [4]
p,water[J/gK]=4.2174−3.176894·10−3T+8.574342·10−5T2−9.3402·10−7T3+3.94926·10−9T4
(3)
(fitted to a fourth order polynomial in temperature [°C]), cp,buffer can be determined properly, if necessary. As long as no absolute values of heat capacity are required, but only transition parameters such as enthalpies or entropies are of interest, approximate values for the specific volumes may be employed. Frequently mean values of vprotein = 0.74 ml/g and vbuffer ≈ 1 ml/g have been used. However, in general it is preferable to determine experimentally the variation with temperature of both specific volumes directly [5,6] or take the individual values from data collections [7]. The specific volume of water is given by the following expression [8]
water[ml/g]=(1+16.87985·10−3T)/(0.9998395+16.945176·10−3T−7.9870401·10−6T2−46.170461·10−9T3+105.56302·10−12T4−280.54253·10−15T5).
(4)
3 THERMODYNAMIC ANALYSIS OF HEAT CAPACITY CURVES
In this section heat capacity is interpreted in a classical thermodynamical way. A more general statistical thermodynamical analysis in a later section will show some differences in interpretation, which renders the DSC method an even more powerful tool in the investigation of protein folding.
3.1 The shape of heat capacity curves
In the simplest case a heat capacity curve of a protein consists of three parts. There are two regions showing roughly a linear temperature dependence of Cp separated by a peak (Figure 1). This peak reflects a first order transition between the two common states of proteins, the so-called native and the denatured state. The native state is the biologically functional state which is populated at physiological conditions. It is also characterised by a well defined three-dimensional structure. In contrast the denatured state has no defined single structure and lacks biological function. The transition region is marked by a heat absorption peak. Its stepwise integrated area has been assumed traditionally to be proportional to the fraction of denatured molecules or equivalently to the population shift. The midpoint temperature of the transition is called T1/2 and has been traditionally defined as the temperature at which 50% of the molecules have been denatured.
3.2 Protein stability
In the present survey protein stability will be defined thermodynamically [9]. Alternatively for other purposes it may be useful to characterise protein stability by the time during which a protein population shows biological activity. Such a criterion is not based on thermodynamic grounds but is rather a question of irreversible kinetics. Therefore we shall refer in this discussion to protein stability in the strict thermodynamic manner by using the standard Gibbs energy change of unfolding NDG0(T) as a quantitative measure of protein stability.
The use of NDG0(T) as a quantitative measure of stability implies reversible experimental conditions. Therefore measurements have to be optimised to exclude the occurrence of irreversibility. Two mayor causes of irreversibility can be distinguished. First, for the establishment of equilibrium conditions the scan rate must be slow compared to the folding kinetics [10,11]. Otherwise the Cp(T)-curve will become distorted. Second, reversible unfolding may be perturbed by an irreversible step following unfolding, if the heating rate is too slow compared with the rate of the irreversible reaction. Interference by such a process can be avoided, if the measurement is completed before a significant amount of the irreversibly misfolded state has accumulated [12-14], The proper choice of the scan rate is therefore dictated by the intrinsic folding properties of the protein but also by the response time of the DSC instrument [15]. These constraints may lead to both an upper and lower limit of the heating rate.
The quantitative description of the transition curve shown in Figure 1 can be accomplished in the following manner. The overall excess heat contribution NDH0(T1/2) of the unfolding transition is represented by the area of the peak, since thermodynamically the heat capacity at constant pressure is defined by the equation
p=(∂H∂T)p.
(5)
Furthermore this means that the heat capacity difference between two states N and D, given by equation...
| Erscheint lt. Verlag | 13.12.1999 |
|---|---|
| Sprache | englisch |
| Themenwelt | Naturwissenschaften ► Biologie ► Biochemie |
| Naturwissenschaften ► Chemie ► Analytische Chemie | |
| Naturwissenschaften ► Chemie ► Physikalische Chemie | |
| Naturwissenschaften ► Physik / Astronomie ► Thermodynamik | |
| Technik | |
| ISBN-10 | 0-08-053569-0 / 0080535690 |
| ISBN-13 | 978-0-08-053569-2 / 9780080535692 |
| Haben Sie eine Frage zum Produkt? |
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