Description

Book Synopsis


Table of Contents

Foreword xix

Acknowledgments xxi

Abbreviations xxiii

Book Navigation xxix

Part I Understanding Cell Culture 1

1. Introduction 3

1.1 Terminology 3

1.2 Historical Development 4

1.3 Applications 12

1.4 Advantages of Tissue Culture 13

1.5 Limitations of Tissue Culture 15

References 18

2. Biology of Cultured Cells 23

2.1 The Culture Environment 23

2.2 Cell Adhesion 23

2.3 Cell Division 28

2.4 Cell Fate 30

2.5 Cell Death 35

References 36

3. Origin and Evolution of Cultured Cells 39

3.1 Origin of Cultured Cells 39

3.2 Evolution of Cell Lines 40

3.3 Changes in Genotype 43

3.4 Changes in Phenotype 46

3.5 Senescence and Immortalization 48

Minireview M3.1 Senescence and Immortalization 48

3.6 Transformation 50

3.7 Conclusions: Origin and Evolution 58

References 58

Part II Laboratory and Regulatory Requirements 63

4. Laboratory Design and Layout 65

4.1 Design Requirements 65

4.2 Layout of Laboratory Areas 74

4.3 Disaster and Contingency Planning 80

References 83

5. Equipment and Materials 85

5.1 Sterile Handling Area Equipment 85

5.2 Imaging and Analysis Equipment 97

5.3 Incubation Equipment 99

5.4 Preparation and Washup Equipment 104

5.5 Cold Storage Equipment 107

References 109

6. Safety and Bioethics 111

6.1 Laboratory Safety 111

6.2 Hazards in Tissue Culture Laboratories 117

6.3 Biosafety 121

6.4 Bioethics 129

References 132

7. Reproducibility and Good Cell Culture Practice 137

7.1 Reproducibility 137

7.2 Good Practice Requirements 141

7.3 Cell Line Provenance 145

7.4 Validation Testing 146

7.5 Quality Assurance (QA) 148

7.6 Replicate Sampling 150

References 151

Part III Medium and Substrate Requirements 155

8. Culture Vessels and Substrates 157

8.1 Attachment and Growth Requirements 157

8.2 Substrate Materials 158

8.3 Substrate Treatments 159

8.4 Feeder Layers 163

8.5 Choice of Culture Vessel 164

8.6 Application-Specific Vessels 170

References 173

9. Defined Media and Supplements 177

9.1 Medium Development 177

9.2 Physicochemical Properties 177

9.3 Balanced Salt Solutions 185

9.4 Media Formulations 186

9.5 Serum 189

9.6 Other Media Supplements 191

9.7 Choice of Complete Medium 191

9.8 Storage of Medium and Serum 194

Suppliers 194

References 194

10. Serum-Free Media 199

10.1 Rationale for Serum-Free Medium 199

10.2 Development of Serum-Free Medium 201

10.3 Serum-Free Media Formulations 202

10.4 Serum-Free Supplements 203

10.5 Serum Replacements 209

10.6 Use of Serum-Free Medium 209

10.7 Xeno-Free Media 213

10.8 Animal Product-Free Media 214

10.9 Conclusions: Serum-Free Media 214

Suppliers 214

References 215

11. Preparation and Sterilization 219

11.1 Terminology: Preparation 219

11.2 Sterilization Methods 220

11.3 Glassware 224

Protocol P11.1 Preparation and Sterilization of Glassware 224

11.4 Other Laboratory Apparatus 229

11.5 Water 229

11.6 Media and Other Reagents 233

11.7 Sterile Filtration 238

11.8 Medium Testing 242

Suppliers 247

References 247

Part IV Handling Cultures 249

12. Aseptic Technique 251

12.1 Objectives of Aseptic Technique 251

12.2 Elements of Aseptic Environment 252

12.3 Sterile Handling 258

12.4 Good Aseptic Technique 260

12.5 Controlling Equipment Contamination 265

Suppliers 267

References 267

13. Primary Culture 269

13.1 Rationale for Primary Culture 269

13.2 Initiation of Primary Culture 270

13.3 Tissue Acquisition and Isolation 274

13.4 Primary Explantation 281

Protocol P13.3 Culture of Primary Explants 281

13.5 Enzymatic Disaggregation 283

13.6 Mechanical Disaggregation 290

Protocol P13.7 Mechanical Disaggregation by Sieving 291

13.7 Enrichment of Viable Cells 292

Protocol P13.8 Enrichment of Viable Cells 292

13.8 Record Keeping for Primary Culture 293

13.9 Conclusions: Primary Culture 294

Suppliers 294

References 294

14. Subculture and Cell Lines 297

14.1 Terminology: Cell Line and Subculture 297

14.2 Initiating a Cell Line 298

14.3 Choosing a Cell Line 300

14.4 Maintaining a Cell Line 304

14.5 Replacing Medium (Feeding) 309

14.6 Subculture (Passaging) 312

14.7 Maintaining Suspension Cultures 320

14.8 Serum-Free Subculture 322

14.9 Record Keeping for Cell Lines 323

Suppliers 324

References 325

15. Cryopreservation and Banking 327

15.1 Principles of Cryopreservation 327

15.2 Apparatus for Cryopreservation 329

15.3 Requirements for Cryopreservation 335

15.4 Cryopreservation Procedures 336

15.5 Cell Banking Procedures 341

15.6 Cell Repositories 342

15.7 Record Keeping for Frozen Stocks 345

15.8 Transporting Cells 347

Suppliers 348

References 348

Part V Validation and Characterization 351

16. Microbial Contamination 353

16.1 Sources of Contamination 353

16.2 Management of Contamination 359

Protocol P16.1 Disposal of Contaminated Cultures 360

16.3 Visible Microbial Contamination 361

16.4 Mycoplasma Contamination 364

16.5 Viral Contamination 373

16.6 Dealing with Persistent Contamination 376

Suppliers 376

References 376

17. Cell Line Misidentification and Authentication 381

17.1 Terminology: Cross-Contamination, Misidentification, and Authentication 381

17.2 Misidentified Cell Lines 382

17.3 Cell Line Authentication 386

17.4 Authentication of Challenging Samples 401

17.5 Conclusions: Authentication 403

Suppliers 403

References 403

18. Cell Line Characterization 409

18.1 Priorities and Essential Characterization 409

18.2 Genotype-Based Characterization 416

18.3 Phenotype-Based Characterization 419

18.4 Cell Imaging 423

18.5 Cell Staining 428

Suppliers 430

References 430

19. Quantitation and Growth Kinetics 437

19.1 Cell Counting 437

19.3 Cell Proliferation 450

19.4 Cloning Efficiency 456

19.5 DNA Synthesis 460

19.6 Cell Cycle Analysis 461

Suppliers 461

References 461

Part VI Physical and Genetic Manipulation 465

20. Cell Cloning and Selection 467

20.1 Terminology: Cloning and Selection 467

20.2 Cloning by Limiting Dilution 468

20.3 Cloning in Suspension 473

20.4 Selection of Clones 477

20.5 Replica Plating 480

20.6 Stimulation of Cloning Efficiency 481

20.7 Selective Culture Conditions 485

20.8 Conclusions: Cloning and Selection 487

Suppliers 487

References 487

21. Cell Separation and Sorting 491

21.1 Cell Density and Isopycnic Centrifugation 491

21.2 Cell Size and Sedimentation Velocity 495

21.3 Magnetic Separation and Sorting 496

Protocol P21.2 Magnet-Activated Cell Sorting (MACS) 499

21.4 Fluorescence-Activated Cell Sorting (FACS) 500

21.5 Microfluidic Sorting 502

Minireview M21.1 Microfluidic Cell Culture 503

21.6 Conclusions: Sorting and Separation 505

Suppliers 505

References 505

22. Genetic Modification and Immortalization 509

22.1 Gene Delivery 509

22.2 Gene Editing 517

22.3 Immortalization 523

22.4 Screening and Artifacts 526

Suppliers 528

References 528

Part VII Stem Cells and Differentiated Cells 535

23. Culture of Stem Cells 537

23.1 Terminology: Stem Cells 537

23.2 Embryonic Stem Cells (ESCs) 540

23.3 Induction of Pluripotency 545

Protocol P23.1 Generation of iPSCs Using Sendai Viral Vectors 547

23.4 Human Pluripotent Stem Cell (hPSC) Lines 549

23.5 Perinatal Stem Cells 556

23.6 Adult Stem Cells 557

23.7 Stem Cell Characterization and Banking 558

23.8 Conclusions: Culture of Stem Cells 560

Suppliers 561

References 561

24. Culture of Specific Cell Types 567

24.1 Specialized Cells and Their Availability 567

24.2 Epithelial Cells 572

24.3 Mesenchymal Cells 577

24.4 Neuroectodermal Cells 580

24.5 Hematopoietic Cells 581

24.6 Culture of Cells from Poikilotherms 585

Suppliers 587

References 587

25. Culture of Tumor Cells 593

25.1 Challenges of Tumor Cell Culture 593

25.2 Primary Culture of Tumor Cells 594

25.3 Development of Tumor Cell Lines 596

25.4 Selective Culture of Tumor Cells 599

25.5 Specific Tumor Types 603

25.6 Cancer Stem Cells (CSCs) 606

Minireview M25.1 Culture of Cancer Stem Cells 606

Suppliers 608

References 608

26. Differentiation 615

26.1 In Vitro Models of Differentiation 615

26.2 Differentiation Status in Culture 617

26.3 Induction of Differentiation 620

26.4 Practical Aspects 628

26.5 Ongoing Challenges 629

Suppliers 631

References 631

Part VIII Model Environments and Applications 639

27. Three-Dimensional Culture 641

27.1 Terminology: 3D Culture 641

27.2 Technologies for 3D Culture 643

Minireview M27.1 Advances in Technologies Enabling 3D Cell Culture and the Formation of Tissue-Like Architecture In Vitro 643

27.3 Benefits and Limitations of 3D Culture 646

27.4 Scaffold-Free 3D Culture Systems 647

27.5 Scaffold-Based 3D Culture Systems 652

27.6 Organoid Culture 659

27.7 Organotypic Culture 660

27.8 Organ Culture 662

27.9 Characterization of 3D Cultures 662

Suppliers 663

References 663

28. Scale-Up and Automation 669

28.1 Terminology: Scale-Up and Bioreactors 669

28.2 Scale-Up in Suspension 671

28.3 Scale-Up in Monolayer 677

28.4 Monitoring and Process Control 685

28.5 Scale-Up for Manufacture 688

Minireview M28.1 Culture Scale-Up and Bioreactors 688

28.6 High-Throughput Screening 691

28.7 Automation and Bioprinting 691

Suppliers 696

References 696

29. Toxicity Testing 701

29.1 In Vitro Toxicity Testing 701

29.2 Cytotoxicity Assays 704

29.3 Genotoxicity Assays 715

29.4 Carcinogenicity Assays 716

29.5 Advanced Models for Toxicity Testing 716

Suppliers 719

References 719

Part IX Teaching and Troubleshooting 725

30. Training 727

30.1 Training Principles 727

30.2 Training Programs 729

References 731

31. Problem Solving 733

31.1 Microbial Contamination 733

31.2 Cross-Contamination and Misidentification 737

31.3 Chemical Contamination 738

31.4 Slow Cell Growth 738

31.5 Abnormal Cell Appearance 740

31.6 Problems with Materials 741

31.7 Problems with Primary Culture 744

31.8 Problems with Feeding or Subculture 746

31.9 Problems with Cryopreservation 748

31.10 Problems with Cloning 750

References 752

32. In Conclusion 753

Appendix A Glossary 755

Appendix B Calculations and Preparation of Reagents 761

Calculations 761

Counting Cells with a Hemocytometer 761

Dilution of a Cell Suspension 761

Population Doubling Level (PDL) 761

Molarity 762

Percentages and Dilutions 762

Pressure 762

Rotor Speed (rpm to g) 762

Preparation of Reagents 762

Acetic Acid: Methanol 762

Agar (2.5%) 762

Alcohol (70%) 762

Bacto Peptone (5%) 763

Balanced Salt Solutions 763

Carboxymethylcellulose (CMC; 4%) 763

Chick Embryo Extract 763

Collagenase 763

Collection Medium 763

Crystal Violet (0.1%) 764

Dexamethasone (1 mg/ml) 764

Dissection Balanced Salt Solution (DBSS) 764

Dulbecco’s Phosphate-Buffered Saline Without Ca2+ and Mg2+ (DPBS-A) 764

EDTA (10 mM in DPBS-A) 764

EGTA 764

Erythrosin B 764

Gelatin (1%) 765

Giemsa Stain 765

Glucose (20%) 765

Glutamine 200 mM 765

Hanks’s Balanced Salt Solution (HBSS) 765

HAT Medium 765

HB Medium 765

HEPES 765

Hoechst 33258 766

Media 766

2-Mercaptoethanol (𝛽-Mercaptoethanol; 0.1 M) 766

Methylcellulose (Methocel, 1.6%) 766

Mitomycin C (100 μg/ml) 766

MTT (50 mg/ml) 766

N2 Supplement 766

N2B27 Medium 767

Naphthalene Black (Amido Black; 1%) 767

Non-essential Amino Acids (NEAA, 100×) 767

Paraformaldehyde (4%) 767

Trypan Blue (0.4%) 767

Trypsin (2.5%) 768

Versene 768

Suppliers 768

References 768

Appendix C Media Formulations 769

References 779

Index 781

Freshneys Culture of Animal Cells

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    Order before 4pm today for delivery by Mon 27 Jul 2026.

    A Hardback by Amanda Capes-Davis, R. Ian Freshney

      Trusted by thousands of customers. See 2,385+ Customer Reviews

      View other formats and editions of Freshneys Culture of Animal Cells by Amanda Capes-Davis

      Publisher: John Wiley and Sons Ltd
      Publication Date: 13/05/2021
      ISBN13: 9781119513018, 978-1119513018
      ISBN10: 1119513014

      Description

      Book Synopsis


      Table of Contents

      Foreword xix

      Acknowledgments xxi

      Abbreviations xxiii

      Book Navigation xxix

      Part I Understanding Cell Culture 1

      1. Introduction 3

      1.1 Terminology 3

      1.2 Historical Development 4

      1.3 Applications 12

      1.4 Advantages of Tissue Culture 13

      1.5 Limitations of Tissue Culture 15

      References 18

      2. Biology of Cultured Cells 23

      2.1 The Culture Environment 23

      2.2 Cell Adhesion 23

      2.3 Cell Division 28

      2.4 Cell Fate 30

      2.5 Cell Death 35

      References 36

      3. Origin and Evolution of Cultured Cells 39

      3.1 Origin of Cultured Cells 39

      3.2 Evolution of Cell Lines 40

      3.3 Changes in Genotype 43

      3.4 Changes in Phenotype 46

      3.5 Senescence and Immortalization 48

      Minireview M3.1 Senescence and Immortalization 48

      3.6 Transformation 50

      3.7 Conclusions: Origin and Evolution 58

      References 58

      Part II Laboratory and Regulatory Requirements 63

      4. Laboratory Design and Layout 65

      4.1 Design Requirements 65

      4.2 Layout of Laboratory Areas 74

      4.3 Disaster and Contingency Planning 80

      References 83

      5. Equipment and Materials 85

      5.1 Sterile Handling Area Equipment 85

      5.2 Imaging and Analysis Equipment 97

      5.3 Incubation Equipment 99

      5.4 Preparation and Washup Equipment 104

      5.5 Cold Storage Equipment 107

      References 109

      6. Safety and Bioethics 111

      6.1 Laboratory Safety 111

      6.2 Hazards in Tissue Culture Laboratories 117

      6.3 Biosafety 121

      6.4 Bioethics 129

      References 132

      7. Reproducibility and Good Cell Culture Practice 137

      7.1 Reproducibility 137

      7.2 Good Practice Requirements 141

      7.3 Cell Line Provenance 145

      7.4 Validation Testing 146

      7.5 Quality Assurance (QA) 148

      7.6 Replicate Sampling 150

      References 151

      Part III Medium and Substrate Requirements 155

      8. Culture Vessels and Substrates 157

      8.1 Attachment and Growth Requirements 157

      8.2 Substrate Materials 158

      8.3 Substrate Treatments 159

      8.4 Feeder Layers 163

      8.5 Choice of Culture Vessel 164

      8.6 Application-Specific Vessels 170

      References 173

      9. Defined Media and Supplements 177

      9.1 Medium Development 177

      9.2 Physicochemical Properties 177

      9.3 Balanced Salt Solutions 185

      9.4 Media Formulations 186

      9.5 Serum 189

      9.6 Other Media Supplements 191

      9.7 Choice of Complete Medium 191

      9.8 Storage of Medium and Serum 194

      Suppliers 194

      References 194

      10. Serum-Free Media 199

      10.1 Rationale for Serum-Free Medium 199

      10.2 Development of Serum-Free Medium 201

      10.3 Serum-Free Media Formulations 202

      10.4 Serum-Free Supplements 203

      10.5 Serum Replacements 209

      10.6 Use of Serum-Free Medium 209

      10.7 Xeno-Free Media 213

      10.8 Animal Product-Free Media 214

      10.9 Conclusions: Serum-Free Media 214

      Suppliers 214

      References 215

      11. Preparation and Sterilization 219

      11.1 Terminology: Preparation 219

      11.2 Sterilization Methods 220

      11.3 Glassware 224

      Protocol P11.1 Preparation and Sterilization of Glassware 224

      11.4 Other Laboratory Apparatus 229

      11.5 Water 229

      11.6 Media and Other Reagents 233

      11.7 Sterile Filtration 238

      11.8 Medium Testing 242

      Suppliers 247

      References 247

      Part IV Handling Cultures 249

      12. Aseptic Technique 251

      12.1 Objectives of Aseptic Technique 251

      12.2 Elements of Aseptic Environment 252

      12.3 Sterile Handling 258

      12.4 Good Aseptic Technique 260

      12.5 Controlling Equipment Contamination 265

      Suppliers 267

      References 267

      13. Primary Culture 269

      13.1 Rationale for Primary Culture 269

      13.2 Initiation of Primary Culture 270

      13.3 Tissue Acquisition and Isolation 274

      13.4 Primary Explantation 281

      Protocol P13.3 Culture of Primary Explants 281

      13.5 Enzymatic Disaggregation 283

      13.6 Mechanical Disaggregation 290

      Protocol P13.7 Mechanical Disaggregation by Sieving 291

      13.7 Enrichment of Viable Cells 292

      Protocol P13.8 Enrichment of Viable Cells 292

      13.8 Record Keeping for Primary Culture 293

      13.9 Conclusions: Primary Culture 294

      Suppliers 294

      References 294

      14. Subculture and Cell Lines 297

      14.1 Terminology: Cell Line and Subculture 297

      14.2 Initiating a Cell Line 298

      14.3 Choosing a Cell Line 300

      14.4 Maintaining a Cell Line 304

      14.5 Replacing Medium (Feeding) 309

      14.6 Subculture (Passaging) 312

      14.7 Maintaining Suspension Cultures 320

      14.8 Serum-Free Subculture 322

      14.9 Record Keeping for Cell Lines 323

      Suppliers 324

      References 325

      15. Cryopreservation and Banking 327

      15.1 Principles of Cryopreservation 327

      15.2 Apparatus for Cryopreservation 329

      15.3 Requirements for Cryopreservation 335

      15.4 Cryopreservation Procedures 336

      15.5 Cell Banking Procedures 341

      15.6 Cell Repositories 342

      15.7 Record Keeping for Frozen Stocks 345

      15.8 Transporting Cells 347

      Suppliers 348

      References 348

      Part V Validation and Characterization 351

      16. Microbial Contamination 353

      16.1 Sources of Contamination 353

      16.2 Management of Contamination 359

      Protocol P16.1 Disposal of Contaminated Cultures 360

      16.3 Visible Microbial Contamination 361

      16.4 Mycoplasma Contamination 364

      16.5 Viral Contamination 373

      16.6 Dealing with Persistent Contamination 376

      Suppliers 376

      References 376

      17. Cell Line Misidentification and Authentication 381

      17.1 Terminology: Cross-Contamination, Misidentification, and Authentication 381

      17.2 Misidentified Cell Lines 382

      17.3 Cell Line Authentication 386

      17.4 Authentication of Challenging Samples 401

      17.5 Conclusions: Authentication 403

      Suppliers 403

      References 403

      18. Cell Line Characterization 409

      18.1 Priorities and Essential Characterization 409

      18.2 Genotype-Based Characterization 416

      18.3 Phenotype-Based Characterization 419

      18.4 Cell Imaging 423

      18.5 Cell Staining 428

      Suppliers 430

      References 430

      19. Quantitation and Growth Kinetics 437

      19.1 Cell Counting 437

      19.3 Cell Proliferation 450

      19.4 Cloning Efficiency 456

      19.5 DNA Synthesis 460

      19.6 Cell Cycle Analysis 461

      Suppliers 461

      References 461

      Part VI Physical and Genetic Manipulation 465

      20. Cell Cloning and Selection 467

      20.1 Terminology: Cloning and Selection 467

      20.2 Cloning by Limiting Dilution 468

      20.3 Cloning in Suspension 473

      20.4 Selection of Clones 477

      20.5 Replica Plating 480

      20.6 Stimulation of Cloning Efficiency 481

      20.7 Selective Culture Conditions 485

      20.8 Conclusions: Cloning and Selection 487

      Suppliers 487

      References 487

      21. Cell Separation and Sorting 491

      21.1 Cell Density and Isopycnic Centrifugation 491

      21.2 Cell Size and Sedimentation Velocity 495

      21.3 Magnetic Separation and Sorting 496

      Protocol P21.2 Magnet-Activated Cell Sorting (MACS) 499

      21.4 Fluorescence-Activated Cell Sorting (FACS) 500

      21.5 Microfluidic Sorting 502

      Minireview M21.1 Microfluidic Cell Culture 503

      21.6 Conclusions: Sorting and Separation 505

      Suppliers 505

      References 505

      22. Genetic Modification and Immortalization 509

      22.1 Gene Delivery 509

      22.2 Gene Editing 517

      22.3 Immortalization 523

      22.4 Screening and Artifacts 526

      Suppliers 528

      References 528

      Part VII Stem Cells and Differentiated Cells 535

      23. Culture of Stem Cells 537

      23.1 Terminology: Stem Cells 537

      23.2 Embryonic Stem Cells (ESCs) 540

      23.3 Induction of Pluripotency 545

      Protocol P23.1 Generation of iPSCs Using Sendai Viral Vectors 547

      23.4 Human Pluripotent Stem Cell (hPSC) Lines 549

      23.5 Perinatal Stem Cells 556

      23.6 Adult Stem Cells 557

      23.7 Stem Cell Characterization and Banking 558

      23.8 Conclusions: Culture of Stem Cells 560

      Suppliers 561

      References 561

      24. Culture of Specific Cell Types 567

      24.1 Specialized Cells and Their Availability 567

      24.2 Epithelial Cells 572

      24.3 Mesenchymal Cells 577

      24.4 Neuroectodermal Cells 580

      24.5 Hematopoietic Cells 581

      24.6 Culture of Cells from Poikilotherms 585

      Suppliers 587

      References 587

      25. Culture of Tumor Cells 593

      25.1 Challenges of Tumor Cell Culture 593

      25.2 Primary Culture of Tumor Cells 594

      25.3 Development of Tumor Cell Lines 596

      25.4 Selective Culture of Tumor Cells 599

      25.5 Specific Tumor Types 603

      25.6 Cancer Stem Cells (CSCs) 606

      Minireview M25.1 Culture of Cancer Stem Cells 606

      Suppliers 608

      References 608

      26. Differentiation 615

      26.1 In Vitro Models of Differentiation 615

      26.2 Differentiation Status in Culture 617

      26.3 Induction of Differentiation 620

      26.4 Practical Aspects 628

      26.5 Ongoing Challenges 629

      Suppliers 631

      References 631

      Part VIII Model Environments and Applications 639

      27. Three-Dimensional Culture 641

      27.1 Terminology: 3D Culture 641

      27.2 Technologies for 3D Culture 643

      Minireview M27.1 Advances in Technologies Enabling 3D Cell Culture and the Formation of Tissue-Like Architecture In Vitro 643

      27.3 Benefits and Limitations of 3D Culture 646

      27.4 Scaffold-Free 3D Culture Systems 647

      27.5 Scaffold-Based 3D Culture Systems 652

      27.6 Organoid Culture 659

      27.7 Organotypic Culture 660

      27.8 Organ Culture 662

      27.9 Characterization of 3D Cultures 662

      Suppliers 663

      References 663

      28. Scale-Up and Automation 669

      28.1 Terminology: Scale-Up and Bioreactors 669

      28.2 Scale-Up in Suspension 671

      28.3 Scale-Up in Monolayer 677

      28.4 Monitoring and Process Control 685

      28.5 Scale-Up for Manufacture 688

      Minireview M28.1 Culture Scale-Up and Bioreactors 688

      28.6 High-Throughput Screening 691

      28.7 Automation and Bioprinting 691

      Suppliers 696

      References 696

      29. Toxicity Testing 701

      29.1 In Vitro Toxicity Testing 701

      29.2 Cytotoxicity Assays 704

      29.3 Genotoxicity Assays 715

      29.4 Carcinogenicity Assays 716

      29.5 Advanced Models for Toxicity Testing 716

      Suppliers 719

      References 719

      Part IX Teaching and Troubleshooting 725

      30. Training 727

      30.1 Training Principles 727

      30.2 Training Programs 729

      References 731

      31. Problem Solving 733

      31.1 Microbial Contamination 733

      31.2 Cross-Contamination and Misidentification 737

      31.3 Chemical Contamination 738

      31.4 Slow Cell Growth 738

      31.5 Abnormal Cell Appearance 740

      31.6 Problems with Materials 741

      31.7 Problems with Primary Culture 744

      31.8 Problems with Feeding or Subculture 746

      31.9 Problems with Cryopreservation 748

      31.10 Problems with Cloning 750

      References 752

      32. In Conclusion 753

      Appendix A Glossary 755

      Appendix B Calculations and Preparation of Reagents 761

      Calculations 761

      Counting Cells with a Hemocytometer 761

      Dilution of a Cell Suspension 761

      Population Doubling Level (PDL) 761

      Molarity 762

      Percentages and Dilutions 762

      Pressure 762

      Rotor Speed (rpm to g) 762

      Preparation of Reagents 762

      Acetic Acid: Methanol 762

      Agar (2.5%) 762

      Alcohol (70%) 762

      Bacto Peptone (5%) 763

      Balanced Salt Solutions 763

      Carboxymethylcellulose (CMC; 4%) 763

      Chick Embryo Extract 763

      Collagenase 763

      Collection Medium 763

      Crystal Violet (0.1%) 764

      Dexamethasone (1 mg/ml) 764

      Dissection Balanced Salt Solution (DBSS) 764

      Dulbecco’s Phosphate-Buffered Saline Without Ca2+ and Mg2+ (DPBS-A) 764

      EDTA (10 mM in DPBS-A) 764

      EGTA 764

      Erythrosin B 764

      Gelatin (1%) 765

      Giemsa Stain 765

      Glucose (20%) 765

      Glutamine 200 mM 765

      Hanks’s Balanced Salt Solution (HBSS) 765

      HAT Medium 765

      HB Medium 765

      HEPES 765

      Hoechst 33258 766

      Media 766

      2-Mercaptoethanol (𝛽-Mercaptoethanol; 0.1 M) 766

      Methylcellulose (Methocel, 1.6%) 766

      Mitomycin C (100 μg/ml) 766

      MTT (50 mg/ml) 766

      N2 Supplement 766

      N2B27 Medium 767

      Naphthalene Black (Amido Black; 1%) 767

      Non-essential Amino Acids (NEAA, 100×) 767

      Paraformaldehyde (4%) 767

      Trypan Blue (0.4%) 767

      Trypsin (2.5%) 768

      Versene 768

      Suppliers 768

      References 768

      Appendix C Media Formulations 769

      References 779

      Index 781

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