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DNA Repair Protocols Daryl S. Henderson

DNA Repair Protocols By Daryl S. Henderson

DNA Repair Protocols by Daryl S. Henderson


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Summary

The field of eukaryotic DNA repair is enjoying a period of remarkable growth and discovery, fueled by technological advances in molecular bi- ogy, protein biochemistry, and genetics.

DNA Repair Protocols Summary

DNA Repair Protocols by Daryl S. Henderson

The field of eukaryotic DNA repair is enjoying a period of remarkable growth and discovery, fueled by technological advances in molecular bi- ogy, protein biochemistry, and genetics. Notable achievements include the molecular cloning of multiple genes associated with classical human repair disorders, such as xeroderma pigmentosum, Cockayne syndrome, and ataxia telangiectasia; elucidation of the core reaction of nucleotide excision repair (NER); the discovery that certain NER proteins participate not only in repair, but also in transcription; recognition of the crucial role played by mismatch repair processes in maintenance of genome stability and avoidance of cancer; the findings that the tumor suppressor protein p53 is mutated in many types of cancer, and has a key role in directing potentially malignant, genotoxin-d- aged cells towards an apoptotic fate; and the discovery and elaboration of DNA damage (and replication) checkpoints, which placed repair phenomen- ogy firmly within a cell-cycle context. Of course, much remains to be learned about DNA repair. To that end, DNA Repair Protocols: Eukaryotic Systems is about the tools and techniques that have helped propel the DNA repair field into the mainstream of biological research. DNA Repair Protocols: Eukaryotic Systems provides detailed, step-- step instructions for studying manifold aspects of the eukaryotic response to genomic injury. The majority of chapters describe methods for analyzing DNA repair processes in mammalian cells. However, many of those techniques can be applied with only minor modification to other systems, and vice versa.

DNA Repair Protocols Reviews

"...a comprehensive series of technique-oriented chapters focusing on eukaryotic DNA repair methodology. ...this text succeeds admirably...The scope of the text is fairly broad and encompasses not only in vitro biochemistry and enzymology, but also cell biology and genetics and even signal transduction....In vitro biochemical assays are well covered,...A particularly nice feature of the book is that the chapters have undergone uniform editing and formatting. All provide a nice overview of the topic, including a brief review of the pertinent literature, followed by step-by-step methods sections. The methods are clearly presented in annotated outline form with cross referencing and high level of detail. Each chapter has a particularly valuable section at the end, called "Notes" in which the authors present some of the nitty-gritty details and tricks of the trade needed to make the techniques work....Overall, this book should provide a valuable laboratory companion for researchers in the area of DNA repair. It serves to provide useful and readable introductions to various topics, along with techniques protocols sufficient for reproducibility....this text will have substantial appeal to the readers of Radiation Research."-Radiation Research

"The list of authors contains many of the leading scientists within the field...Protocols for most experimental eukaryotic organisms are described, from yeast through plants, worms, flies and frogs to mammals. Another laudable quality of this book is the standardization of the descriptions in Materials and methods. Since (almost) all articles are organized similarly, it is relatively easy to find what you want. Also, technical details have been standardized....At the end of each article , there is a 'Notes' section with detailed explanation of specific technical points. For a novice it is good to be reminded that ethidium bromide is a mutagen and that lids should be loosened before putting flasks in the microwave oven. Iparticularly liked the description, written by the editor, of how to squash Drosophila larvae on a microscope slide by"standing on it with the ball of your foot or your heel. If using the foot method, place the slide (sandwiched in 3 MED MER) on a hard clean floor, cover it carefully with a piece of wood, and stand on that". ...this book keeps up the reputation of the 'Methods in Molecular Biology' series and I would recommend if for labs working with DNA repair, in particular for use by students and technicians."-FEBS Letters

Table of Contents

Mutant Isolation and Gene Cloning.- Isolation of DNA Structure-Dependent Checkpoint Mutants in S. pombe.- Isolating Mutants of the Nematode Caenorhabditis elegans That Are Hypersensitive to DNA-Damaging Agents.- Isolating DNA Repair Mutants of Drosophila melanogaster.- Generation, Identification, and Characterization of Repair-Defective Mutants of Arabidopsis.- Screening for ?-Ray Hypersensitive Mutants of Arabidopsis.- Isolation of Mutagen-Sensitive Chinese Hamster Cell Lines by Replica Plating.- Strategies for Cloning Mammalian DNA Repair Genes.- Novel Complementation Assays for DNA Repair-Deficient Cells.- Recognition and Removal of Inappropriate or Damaged DNA Bases.- The Use of Electrophoretic Mobility Shift Assays to Study DNA Repair.- Mismatch Repair Assay.- Measurement of Activities of Cyclobutane-Pyrimidine-Dimer and (6-4)-Photoproduct Photolyases.- A Dot Blot Immunoassay for UV Photoproducts.- Measurement of UV Radiation-Induced DNA Damage Using Specific Antibodies.- Quantification of Photoproducts in Mammalian Cell DNA Using Radioimmunoassay.- Monitoring Removal of Cyclobutane Pyrimidine Dimers in Arabidopsis.- DNA Damage Quantitation by Alkaline Gel Electrophoresis.- The Comet Assay (Single-Cell Gel Test).- Measuring the Formation and Repair of UV Photoproducts by Ligation-Mediated PCR.- PCR-Based Assays for Strand-Specific Measurement of DNA Damage and Repair I.- PCR-Based Assays for Strand-Specific Measurement of DNA Damage and Repair II.- Gene-Specific and Mitochondrial Repair of Oxidative DNA Damage.- Characterization of DNA Strand Cleavage by Enzymes That Act at Abasic Sites in DNA.- Base Excision Repair Assay Using Xenopus laevis Oocyte Extracts.- In Vitro Base Excision Repair Assay Using Mammalian Cell Extracts.- Nucleotide Excision Repair inSaccharomyces cerevisiae Whole-Cell Extracts.- In Vitro Excision Repair Assay in Schizosaccharomyces pombe.- Nucleotide Excision Repair Assay in Drosophila melanogaster Using Established Cell Lines.- Nucleotide Excision Repair in Nuclear Extracts from Xenopus Oocytes.- Assay for Nucleotide Excision Repair Protein Activity Using Fractionated Cell Extracts and UV-Damaged Plasmid DNA.- Dual-Incision Assays for Nucleotide Excision Repair Using DNA with a Lesion at a Specific Site.- DNA Strand Breakage and Repair.- In Vitro Chemiluminescence Assay to Measure Excision Repair in Cell Extracts.- Physical Monitoring of HO-Induced Homologous Recombination.- Use of P Element Transposons to Study DNA Double-Strand Break Repair in Drosophila melanogaster.- Analyzing Double-Strand Repair Events in Drosophila.- Expression of I-Sce I in Drosophila to Induce DNA Double-Strand Breaks.- Use of I-Sce I to Induce DNA Double-Strand Breaks in Nicotiana.- Chromosomal Double-Strand Breaks Introduced in Mammalian Cells by Expression of I-Sce I Endonuclease.- Induction of DNA Double-Strand Breaks by Electroporation of Restriction Enzymes into Mammalian Cells.- In Vitro Rejoining of Double-Strand Breaks in Genomic DNA.- Extrachromosomal Assay for DNA Double-Strand Break Repair.- Use of Gene Targeting to Study Recombination in Mammalian DNA Repair Mutants.- DNA Damage Tolerance Mechanisms and Regulatory Responses.- Measurement of Low-Frequency DNA Breaks Using Nucleoid Flow Cytometry.- Live Analysis of the Division Cycles in X-Irradiated Drosophila Embryos.- Inhibition of DNA Synthesis by Ionizing Radiation.- Analysis of Inhibition of DNA Replication in Irradiated Cells Using the SV40-Based In Vitro Assay of DNA Replication.- Assays of Bypass Replication of Genotoxic Lesions in Mammalian Disease and Mutant Cell-Free Extracts.- Detection of Chromatin-Bound PCNA in Cultured Cells Following Exposure to DNA-Damaging Agents.- Induction of p53 Protein as a Marker for Ionizing Radiation Exposure In Vivo.- Activation of p53 Protein Function in Response to Cellular Irradiation.- Selective Extraction of Fragmented DNA from Apoptotic Cells for Analysis by Gel Electrophoresis and Identification of Apoptotic Cells by Flow Cytometry.- Detection of DNA Strand Breakage in the Analysis of Apoptosis and Cell Proliferation by Flow and Laser Scanning Cytometry.- Immunoassay for Single-Stranded DNA in Apoptotic Cells.

Additional information

NPB9780896038028
9780896038028
B01GSUM6WK
DNA Repair Protocols by Daryl S. Henderson
New
Hardback
Humana Press Inc.
1999-06-21
642
N/A
Book picture is for illustrative purposes only, actual binding, cover or edition may vary.
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