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• Volume 1
  • Chapter 1: Isolation and Quantification of DNA1
    • Protocol 1: Preparation of Plasmid DNA by Alkaline Lysis with SDS: Minipreps
    • Protocol 2: Preparation of Plasmid DNA by Alkaline Lysis with SDS: Maxipreps
    • Protocol 3: Isolating DNA from Gram-Negative Bacteria (e.g., E. coli)
    • Protocol 4: Precipitation of DNA with Ethanol
    • Protocol 5: Precipitation of DNA with Isopropanol
    • Protocol 6: Concentrating and Desalting Nucleic Acids with Microconcentrators
    • Protocol 7: Concentrating Nucleic Acids by Extraction with Butanol
    • Protocol 8: Preparation of Single-Stranded Bacteriophage M13 DNA by Precipitation with Polyethylene Glycol
    • Protocol 9: Plating Bacteriophage M13
    • Protocol 10: Growing Bacteriophage M13 in Liquid Culture
    • Protocol 11: Preparation of Double-Stranded (Replicative Form) Bacteriophage M13 DNA
    • Protocol 12: Isolation of High-Molecular-Weight DNA Using Organic Solvents to Purify DNA
    • Protocol 13: Isolation of High-Molecular-Weight DNA from Mammalian Cells Using Proteinase K and Phenol
    • Protocol 14: A Single-Step Method for the Simultaneous Preparation of DNA, RNA, and Protein from Cells and Tissues
    • Protocol 15: Preparation of Genomic DNA from Mouse Tails and Other Small Samples
    • Protocol 16: Rapid Isolation of Yeast DNA
    • Protocol 17: Using Ethidium Bromide to Estimate the Amount of DNA in Bands after Electrophoresis through Minigels
    • Protocol 18: Estimating the Concentration of DNA by Fluorometry Using Hoechst 33258
    • Protocol 19: Quantifying DNA in Solution with PicoGreen
    • Panel: Isolation and Quantification of DNA1
    • Panel: DNA Isolation2
    • Panel: Commercial Kits for Purification of DNA3
    • Panel: Quantifying DNA5
    • Panel: Alternative Protocol: Isolation of DNA from Mouse Tails without Extraction by Organic Solvents61
    • Panel: Alternative Protocol: One-Tube Isolation of DNA from Mouse Tails62
    • Panel: DNA Extraction from Formaldehyde-Fixed Tissue Embedded in Paraffin Blocks72
    • Panel: Polyethylene Glycol73
    • Panel: -Complementation74
    • Panel: X-Gal76
    • Panel: Minimizing Damage to Large DNA Molecules77
    • Panel: Spectrophotometry78
  • Chapter 2: Analysis of DNA81
    • Protocol 1: Agarose Gel Electrophoresis
    • Protocol 2: Detection of DNA in Agarose Gels by Staining
    • Protocol 3: Polyacrylamide Gel Electrophoresis
    • Protocol 4: Detection of DNA in Polyacrylamide Gels by Staining
    • Protocol 5: Detection of DNA in Polyacrylamide Gels by Autoradiography
    • Protocol 6: Alkaline Agarose Gel Electrophoresis
    • Protocol 7: Imaging: Autoradiography and Phosphorimaging
    • Protocol 8: Recovery of DNA from Agarose Gels Using Glass Beads
    • Protocol 9: Recovery of DNA from Low-Melting-Temperature Agarose Gels: Organic Extraction
    • Protocol 10: Isolation of DNA Fragments from Polyacrylamide Gels by the Crush and Soak Method
    • Protocol 11: Southern Blotting
    • Protocol 12: Southern Blotting: Simultaneous Transfer of DNA from an Agarose Gel to Two Membranes
    • Protocol 13: Southern Hybridization of Radiolabeled Probes to Nucleic Acids Immobilized on Membranes
    • Panel: Analysis of DNA81
    • Panel: Agarose Gel Electrophoresis82
    • Panel: Analysis of DNA Fragments86
    • Panel: Recovering DNA from Gels87
    • Panel: Southern Blotting88
    • Panel: Additional Protocol: Autoradiography of Alkaline Agarose Gels117
    • Panel: Additional Protocol: Stripping Probes from Membranes150
    • Panel: Formamide and Its Uses in Molecular Cloning153
    • Panel: Rapid Hybridization Buffers155
  • Chapter 3: Cloning and Transformation with Plasmid Vectors157
    • Protocol 1: The Hanahan Method for Preparation and Transformation of Competent E. coli: High-Efficiency Transformation
    • Protocol 2: The Inoue Method for Preparation and Transformation of Competent E. coli: Ultracompetent Cells
    • Protocol 3: Easy Transformation of E. coli: Nanoparticle-Mediated Transformation
    • Protocol 4: Transformation of E. coli by Electroporation
    • Protocol 5: Cloning in Plasmid Vectors: Directional Cloning
    • Protocol 6: Cloning in Plasmid Vectors: Blunt-End Cloning
    • Protocol 7: Dephosphorylation of Plasmid DNA
    • Protocol 8: Attaching Phosphorylated Adaptors/Linkers to Blunt-Ended DNAs
    • Protocol 9: Cloning PCR Products: Addition of Restriction Sites to the Termini of Amplified DNA
    • Protocol 10: Cloning PCR Products: Blunt-End Cloning
    • Protocol 11: Cloning PCR Products: Making T Vectors
    • Protocol 12: Cloning PCR Products: TA Cloning
    • Protocol 13: Cloning PCR Products: TOPO TA Cloning
    • Protocol 14: Screening Bacterial Colonies Using X-Gal and IPTG: -Complementation
    • Panel: Cloning and Transformation with Plasmid Vectors157
    • Panel: Plasmid Vectors158
    • Panel: Transformation159
    • Panel: Alternative Protocol: One-Step Preparation of Competent E. coli: Transformation and Storage of Bacterial Cells in the Same Solution175
    • Panel: Caring for E. coli213
    • Panel: The History of Transformation of Bacteria by DNA217
    • Panel: A Guide to Cloning the Products of Polymerase Chain Reactions218
    • Panel: BioBricks and the Ordered Assembly of DNA Fragments225
    • Panel: TOPO Tools: Creating Linear Expression Constructs with Functional Elements227
    • Panel: Antibiotics229
    • Panel: Adaptors232
    • Panel: Linkers234
    • Panel: Ligation and Ligases235
    • Panel: Condensing and Crowding Reagents240
    • Panel: The Discovery of Restriction Enzymes241
    • Panel: Restriction Enzymes242
    • Panel: Chloramphenicol245
    • Panel: The ccdB Gene247
    • Panel: Bacteriophage 248
    • Panel: Bacteriophage M13249
    • Panel: Plasmids251
    • Panel: Cosmids258
  • Chapter 4: Gateway Recombinational Cloning261
    • Protocol 1: Propagating Gateway Vectors
    • Protocol 2: Generating an ORF Entry Clone and Destination Clone
    • Protocol 3: Using Multisite LR Cloning to Generate a Destination Clone
    • Panel: Gateway Recombinational Cloning261
    • Panel: Basic Principles and Applications of Gateway Cloning262
    • Panel: Disadvantages of Gateway Cloning and Alternative Cloning Systems264
    • Panel: Generating Gateway-Compatible Vectors280
  • Chapter 5: Working with Bacterial Artificial Chromosomes and Other High-Capacity Vectors281
    • Protocol 1: Small-Scale Isolation of BAC DNA and Verification by PCR
    • Protocol 2: Large-Scale Preparation and Linearization of BAC DNA
    • Protocol 3: Examination of BAC DNA Quality and Quantity by Pulsed-Field Gel Electrophoresis
    • Protocol 4: Two-Step BAC Engineering: Preparation of Shuttle Vector DNA
    • Protocol 5: Preparation of the A Homology Arm (A-Box) and B Homology Arm (B-Box)
    • Protocol 6: Cloning of the A and B Homology Arms into the Shuttle Vector
    • Protocol 7: Preparation and Verification of the Recombinant Shuttle Vector
    • Protocol 8: Electroporation of Competent BAC Host Cells with the Recombinant Shuttle Vector
    • Protocol 9: Verification of Cointegrates and Selection of Resolved BAC Clones
    • Protocol 10: One-Step BAC Modification: Preparation of Plasmids
    • Protocol 11: Preparation of the A Homology Arm (A-Box)
    • Protocol 12: Cloning of the A Homology Arm into Reporter-Shuttle Vector
    • Protocol 13: Transformation of the BAC Host with the RecA Vector
    • Protocol 14: Transfer of the Reporter Vector into BAC/RecA Cells and Selection of Cointegrates
    • Protocol 15: Growth of S. cerevisiae and Preparation of DNA
    • Protocol 16: Small-Scale Preparations of Yeast DNA
    • Panel: Working with Bacterial Artificial Chromosomes and Other High-Capacity Vectors281
    • Panel: Development of High-Capacity Vectors: Advantages and Disadvantages282
    • Panel: Working with Bacterial Artificial Chromosomes286
    • Panel: CREloxP338
    • Panel: Using EGFP as a Reporter342
    • Panel: Primer Design for Homology Arms, Cointegration, and Resolution343
    • Panel: Yeast Media344
  • Chapter 6: Extraction, Purification, and Analysis of RNA from Eukaryotic Cells345
    • Protocol 1: Purification of Total RNA from Mammalian Cells and Tissues
    • Protocol 2: Isolation of Total RNA from Zebrafish Embryos and Adults
    • Protocol 3: Total RNA Isolation from Drosophila melanogaster
    • Protocol 4: Total RNA Extraction from Caenorhabditis elegans
    • Protocol 5: Total RNA Extraction from Saccharomyces cerevisiae Using Hot Acid Phenol
    • Protocol 6: Quantifying and Storing RNA
    • Protocol 7: Precipitation of RNA with Ethanol
    • Protocol 8: Removing DNA Contamination from RNA Samples by Treatment with RNase-Free DNase I
    • Protocol 9: Isolation of Poly(A) Messenger RNA Using Magnetic Oligo(dT) Beads
    • Protocol 10: Separation of RNA according to Size: Electrophoresis of RNA through Agarose Gels Containing Formaldehyde
    • Protocol 11: Separation of RNA according to Size: Electrophoresis of RNA through Denaturing Urea Polyacrylamide Gels
    • Protocol 12: Transfer and Fixation of Denatured RNA in Agarose Gels to Membranes
    • Protocol 13: Transfer and Fixation of Denatured RNA in Polyacrylamide Gels to Membranes by Electrophoretic Transfer
    • Protocol 14: Northern Hybridization
    • Protocol 15: Dot and Slot Hybridization of Purified RNA
    • Protocol 16: Mapping RNA with Nuclease S1
    • Protocol 17: Ribonuclease Protection: Mapping RNA with Ribonuclease and Radiolabeled RNA Probes
    • Protocol 18: Analysis of RNA by Primer Extension
    • Panel: Extraction, Purification, and Analysis of RNA from Eukaryotic Cells345
    • Panel: Introduction to the Isolation of Total RNA Using Monophasic Lysis Reagents348
    • Panel: Alternative Protocol: Preparing RNA from Smaller Samples354
    • Panel: Introduction to Hybridization of RNA by Northern Transfer381
    • Panel: Alternative Protocol: Capillary Transfer by Downward Flow406
    • Panel: Introduction to Mapping RNA420
    • Panel: How to Win the Battle with RNase450
    • Panel: Inhibitors of RNases451
    • Panel: Diethylpyrocarbonate452
    • Panel: Nuclease S1454
  • Chapter 7: Polymerase Chain Reaction455
    • Protocol 1: The Basic Polymerase Chain Reaction
    • Protocol 2: Hot Start PCR
    • Protocol 3: Touchdown PCR
    • Protocol 4: PCR Amplification of GC-Rich Templates
    • Protocol 5: Long and Accurate PCR (LA PCR)
    • Protocol 6: Inverse PCR
    • Protocol 7: Nested PCR
    • Protocol 8: Amplification of cDNA Generated by Reverse Transcription of mRNA: Two-Step RT-PCR
    • Protocol 9: Rapid Amplification of Sequences from the 5 Ends of mRNAs: 5-RACE
    • Protocol 10: Rapid Amplification of Sequences from the 3 Ends of mRNAs: 3-RACE
    • Protocol 11: Screening Colonies by PCR
    • Panel: Polymerase Chain Reaction455
    • Panel: The Basic Polymerase Chain Reaction456
    • Panel: Design of Oligonucleotide Primers for Basic PCR462
    • Panel: Detecting, Analyzing, and Quantifying mRNAs464
    • Panel: Contamination in PCR466
    • Panel: Taq DNA Polymerase533
    • Panel: PCR in Theory537
    • Panel: Ribonuclease H538
    • Panel: The dut and ung Genes of E. coli539
    • Panel: Terminal Transferase540
  • Chapter 8: Bioinformatics541
    • Protocol 1: Visualizing Genomic Annotations with the UCSC Genome Browser
    • Protocol 2: Sequence Alignment and Homology Search with BLAST and ClustalW
    • Protocol 3: Designing PCR Primers Using Primer3Plus
    • Protocol 4: Expression Profiling by Microarray and RNA-seq
    • Protocol 5: Mapping Billions of Short Reads to a Reference Genome
    • Protocol 6: Identifying Regions Enriched in a ChIP-seq Data Set (Peak Finding)
    • Protocol 7: Discovering cis-Regulatory Motifs
    • Panel: Bioinformatics541
    • Panel: Introduction to Sequence Alignment and Homology Search554
    • Panel: Introduction to Expression Profiling by Microarray and RNA-seq571
    • Panel: Introduction to Mapping Billions of Short Reads to a Reference Genome588
    • Panel: Introduction to Peak-Finding Algorithms598
    • Panel: Introduction to Motif Finding612
    • Panel: Data Formats625
    • Panel: Algorithms, Portals, and Methods628
• Volume 2
  • Chapter 9: Quantification of DNA and RNA by Real-Time Polymerase Chain Reaction631
    • Protocol 1: Optimizing Primer and Probe Concentrations for Use in Real-Time PCR
    • Protocol 2: Constructing a Standard Curve
    • Protocol 3: Quantification of DNA by Real-Time PCR
    • Protocol 4: Quantification of RNA by Real-Time RT-PCR
    • Protocol 5: Analysis and Normalization of Real-Time PCR Experimental Data
    • Panel: Quantification of DNA and RNA by Real-Time Polymerase Chain Reaction631
    • Panel: Real-Time PCR Chemistries632
    • Panel: Instruments for Real-Time PCR639
    • Panel: Extracting Data from a Real-Time PCR Experiment: Data Analysis and Normalization Methods641
    • Panel: Designing Primers and Probes and Optimizing Conditions for Real-Time PCR643
    • Panel: Constructing a Standard Curve648
    • Panel: Performing Real-Time PCR650
    • Panel: Performing Real-Time RT-PCR650
    • Panel: MIQE Guidelines654
    • Panel: Real-Time PCR Protocols654
    • Panel: Multiplex PCR680
    • Panel: SNP Genotyping681
  • Chapter 10: Nucleic Acid Platform Technologies683
    • Protocol 1: Printing Microarrays
    • Protocol 2: Round A/Round B Amplification of DNA
    • Protocol 3: T7 Linear Amplification of DNA (TLAD) for Nucleosomal and Other DNA < 500 bp
    • Protocol 4: Amplification of RNA
    • Protocol 5: Direct Cyanine-dUTP Labeling of RNA
    • Protocol 6: Indirect Aminoallyl-dUTP Labeling of RNA
    • Protocol 7: Cyanine-dCTP Labeling of DNA Using Klenow
    • Protocol 8: Indirect Labeling of DNA
    • Protocol 9: Blocking Polylysines on Homemade Microarrays
    • Protocol 10: Hybridization to Homemade Microarrays
    • Panel: Nucleic Acid Platform Technologies683
    • Panel: Microarray Applications685
    • Panel: Performing Microarray Experiments688
  • Chapter 11: DNA Sequencing735
    • Protocol 1: Preparing Plasmid Subclones for Capillary Sequencing
    • Protocol 2: Preparing PCR Products for Capillary Sequencing
    • Protocol 3: Cycle-Sequencing Reactions
    • Protocol 4: Whole Genome: Manual Library Preparation
    • Protocol 5: Whole Genome: Automated, Nonindexed Library Preparation
    • Protocol 6: Whole Genome: Automated, Indexed Library Preparation
    • Protocol 7: Preparation of a 3-kb Mate-Pair Library for Illumina Sequencing
    • Protocol 8: Preparation of an 8-kb Mate-Pair Library for Illumina Sequencing
    • Protocol 9: RNA-Seq: RNA Conversion to cDNA and Amplification
    • Protocol 10: Solution-Phase Exome Capture
    • Protocol 11: Automated Size Selection
    • Protocol 12: Library Quantification Using SYBR Green-qPCR
    • Protocol 13: Library Quantification Using PicoGreen Fluorometry
    • Protocol 14: Library Quantification: Fluorometric Quantitation of Double-Stranded or Single-Stranded DNA Samples Using the Qubit System
    • Protocol 15: Preparation of Small-Fragment Libraries for 454 Sequencing
    • Protocol 16: sstDNA Library Capture and emPCR
    • Protocol 17: Roche/454 Sequencer: Executing a Sequencing Run
    • Protocol 18: Validation
    • Protocol 19: Quality Assessment of Sequence Data
    • Protocol 20: Data Analysis
    • Panel: DNA Sequencing735
    • Panel: History of Sanger/Dideoxy DNA Sequencing736
    • Panel: Next-Generation Sequencing742
    • Panel: Overview of Next-Generation Sequencing Instruments752
    • Panel: Sanger Sequencing versus Next-Generation Sequencing: When to Do What?760
    • Panel: Introduction to Protocols761
    • Panel: Additional Protocol: Automated Library Preparation789
    • Panel: Additional Protocol: AMPure Bead Calibration821
    • Panel: Additional Protocol: RNAClean XP Bead Cleanup (before RNA-Seq)830
    • Panel: Additional Protocol: AMPure XP Bead Cleanup840
    • Panel: Additional Protocol: Agarose Gel Size Selection842
    • Panel: Biotin888
    • Panel: Magnetic Beads890
    • Panel: Fragmenting of DNA892
  • Chapter 12: Analysis of DNA Methylation in Mammalian Cells893
    • Protocol 1: DNA Bisulfite Sequencing for Single-Nucleotide-Resolution DNA Methylation Detection
    • Protocol 2: Methylation-Specific PCR for Gene-Specific DNA Methylation Detection
    • Protocol 3: Methyl-Cytosine-Based Immunoprecipitation for DNA Methylation Analysis
    • Protocol 4: High-Throughput Deep Sequencing for Mapping Mammalian DNA Methylation
    • Protocol 5: Roche 454 Clonal Sequencing of Bisulfite-Converted DNA Libraries
    • Protocol 6: Illumina Sequencing of Bisulfite-Converted DNA Libraries
    • Panel: Analysis of DNA Methylation in Mammalian Cells893
    • Panel: DNA Methylation Affects and Reveals Biological Phenomena894
    • Panel: Experimental Approaches for Analysis of DNA Methylation895
    • Panel: Advantages and Limitations of Different Approaches for Analyzing DNA Methylation898
    • Panel: Future Perspectives899
    • Panel: Public Domain Software for Identifying CpG Islands in Promoter and Coding Regions of Mammalian Genes937
    • Panel: Designing Primers for the Amplification of Bisulfite-Converted Product to Perform Bisulfite Sequencing and MS-PCR939
    • Panel: Postsequence Processing of High-Throughput Bisulfite Deep-Sequencing Data940
  • Chapter 13: Preparation of Labeled DNA, RNA, and Oligonucleotide Probes943
    • Protocol 1: Random Priming: Labeling of Purified DNA Fragments by Extension of Random Oligonucleotides
    • Protocol 2: Random Priming: Labeling of DNA by Extension of Random Oligonucleotides in the Presence of Melted Agarose
    • Protocol 3: Labeling of DNA Probes by Nick Translation
    • Protocol 4: Labeling of DNA Probes by Polymerase Chain Reaction
    • Protocol 5: Synthesis of Single-Stranded RNA Probes by In Vitro Transcription
    • Protocol 6: Synthesis of cDNA Probes from mRNA Using Random Oligonucleotide Primers
    • Protocol 7: Radiolabeling of Subtracted cDNA Probes by Random Oligonucleotide Extension
    • Protocol 8: Labeling 3 Termini of Double-Stranded DNA Using the Klenow Fragment of E. coli DNA Polymerase I
    • Protocol 9: Dephosphorylation of DNA Fragments with Alkaline Phosphatase
    • Protocol 10: Phosphorylation of DNA Molecules with Protruding 5-Hydroxyl Termini
    • Protocol 11: Phosphorylation of DNA Molecules with Dephosphorylated Blunt Ends or Recessed 5 Termini
    • Protocol 12: Phosphorylating the 5 Termini of Oligonucleotides Using T4 Polynucleotide Kinase
    • Protocol 13: Labeling the 3 Termini of Oligonucleotides Using Terminal Deoxynucleotidyl Transferase
    • Protocol 14: Labeling of Synthetic Oligonucleotides Using the Klenow Fragment of E. coli DNA Polymerase I
    • Protocol 15: Purification of Labeled Oligonucleotides by Precipitation with Ethanol
    • Protocol 16: Purification of Labeled Oligonucleotides by Size-Exclusion Chromatography
    • Protocol 17: Purification of Labeled Oligonucleotides by Chromatography on a Sep-Pak C₁₈ Column
    • Protocol 18: Hybridization of Oligonucleotide Probes in Aqueous Solutions: Washing in Buffers Containing Quaternary Ammonium Salts
    • Panel: Preparation of Labeled DNA, RNA, and Oligonucleotide Probes943
    • Panel: Radioactive versus Nonradioactive Labeling of Nucleic Acids944
    • Panel: Types of Nonradioactive Detection Systems948
    • Panel: Designing Oligonucleotides for Use as Probes953
    • Panel: Additional Protocol: Asymmetric Probes982
    • Panel: Additional Protocol: Using PCR to Add Promoters for Bacteriophage-Encoded RNA Polymerases to Fragments of DNA991
    • Panel: Alternative Protocol: Synthesizing Nonradiolabeled Probes Using TdT1023
    • Panel: Additional Protocol: Tailing Reaction1024
    • Panel: Additional Protocol: Modifications for Synthesizing Nonradiolabeled Probes1026
    • Panel: Preparation of Stock Solutions of dNTPs1043
    • Panel: E. coli DNA Polymerase I and the Klenow Fragment1044
    • Panel: In Vitro Transcription Systems1050
    • Panel: Alkaline Phosphatase1053
    • Panel: Melting Temperatures1055
  • Chapter 14: Methods for In Vitro Mutagenesis1059
    • Protocol 1: Random Mutagenesis Using Error-Prone DNA Polymerases
    • Protocol 2: Creating Insertions or Deletions Using Overlap Extension PCR Mutagenesis
    • Protocol 3: In Vitro Mutagenesis Using Double-Stranded DNA Templates: Selection of Mutants with DpnI
    • Protocol 4: Altered -Lactamase Selection Approach for Site-Directed Mutagenesis
    • Protocol 5: Oligonucleotide-Directed Mutagenesis by Elimination of a Unique Restriction Site (USE Mutagenesis)
    • Protocol 6: Saturation Mutagenesis by Codon Cassette Insertion
    • Protocol 7: Random Scanning Mutagenesis
    • Protocol 8: Multisite-Directed Mutagenesis
    • Protocol 9: Megaprimer PCR-Based Mutagenesis
    • Panel: Methods for In Vitro Mutagenesis1059
    • Panel: Mutagenesis Approaches1064
    • Panel: Research Goals1065
    • Panel: Commercial Kits1065
    • Panel: Domain Mutagenesis1127
    • Panel: High-Throughput Site-Directed Mutagenesis of Plasmid DNA1128
    • Panel: N⁶-Methyladenine, Dam Methylase, and Methylation-Sensitive Restriction Enzymes1129
  • Chapter 15: Introducing Genes into Cultured Mammalian Cells1131
    • Protocol 1: DNA Transfection Mediated by Cationic Lipid Reagents
    • Protocol 2: Calcium-Phosphate-Mediated Transfection of Eukaryotic Cells with Plasmid DNAs
    • Protocol 3: Calcium-Phosphate-Mediated Transfection of Cells with High-Molecular-Weight Genomic DNA
    • Protocol 4: Transfection Mediated by DEAE-Dextran: High-Efficiency Method
    • Protocol 5: DNA Transfection by Electroporation
    • Protocol 6: Analysis of Cell Viability by the alamarBlue Assay
    • Protocol 7: Analysis of Cell Viability by the Lactate Dehydrogenase Assay
    • Protocol 8: Analysis of Cell Viability by the MTT Assay
    • Panel: Introducing Genes into Cultured Mammalian Cells1131
    • Panel: Transient Versus Stable Transfection1133
    • Panel: Transfection Methods1133
    • Panel: Transfection Controls1133
    • Panel: Optimization and Special Considerations1136
    • Panel: Assessing Cell Viability in Transfected Cell Lines1137
    • Panel: Alternative Protocol: Transfection Using DOTMA and DOGS1145
    • Panel: Additional Protocol: Histochemical Staining of Cell Monolayers for -Galactosidase1148
    • Panel: Alternative Protocol: High-Efficiency Calcium-Phosphate-Mediated Transfection of Eukaryotic Cells with Plasmid DNAs1156
    • Panel: Alternative Protocol: Calcium-Phosphate-Mediated Transfection of Adherent Cells1163
    • Panel: Alternative Protocol: Calcium-Phosphate-Mediated Transfection of Cells Growing in Suspension1165
    • Panel: Alternative Protocol: Transfection Mediated by DEAE-Dextran: Increased Cell Viability1170
    • Panel: Optical Transfection1186
    • Panel: Cotransformation1188
    • Panel: Selective Agents for Stable Transformation1190
    • Panel: Lipofection1194
    • Panel: Linearizing Plasmids before Transfection1197
    • Panel: Transfection of Mammalian Cells with Calcium PhosphateDNA Coprecipitates1198
    • Panel: Chloroquine Diphosphate1200
    • Panel: DEAE-Dextran Transfection1201
    • Panel: Electroporation1203
  • Chapter 16: Introducing Genes into Mammalian Cells: Viral Vectors1209
    • Protocol 1: Construction of Recombinant Adenovirus Genomes by Direct Cloning
    • Protocol 2: Release of the Cloned Recombinant Adenovirus Genome for Rescue and Expansion
    • Protocol 3: Purification of the Recombinant Adenovirus by Cesium Chloride Gradient Centrifugation
    • Protocol 4: Characterization of the Purified Recombinant Adenovirus for Viral Genome Structure by Restriction Enzyme Digestions
    • Protocol 5: Measuring the Infectious Titer of Recombinant Adenovirus Using TCID₅₀ End-Point Dilution and qPCR
    • Protocol 6: Detection Assay for Replication-Competent Adenovirus by Concentration Passage and Real-Time qPCR
    • Protocol 7: Production of rAAVs by Transient Transfection
    • Protocol 8: Purification of rAAVs by Cesium Chloride Gradient Sedimentation
    • Protocol 9: Purification of rAAVs by Iodixanol Gradient Centrifugation
    • Protocol 10: Purification of rAAV2s by Heparin Column Affinity Chromatography
    • Protocol 11: Enrichment of Fully Packaged Virions in Column-Purified rAAV Preparations by Iodixanol Gradient Centrifugation Followed by Anion-Exchange Column Chromatography
    • Protocol 12: Titration of rAAV Genome Copy Number Using Real-Time qPCR
    • Protocol 13: Sensitive Determination of Infectious Titer of rAAVs Using TCID₅₀ End-Point Dilution and qPCR
    • Protocol 14: Analysis of rAAV Sample Morphology Using Negative Staining and High-Resolution Electron Microscopy
    • Protocol 15: Analysis of rAAV Purity Using Silver-Stained SDS-PAGE
    • Protocol 16: Production of High-Titer Retrovirus and Lentivirus Vectors
    • Protocol 17: Titration of Lentivirus Vectors
    • Protocol 18: Monitoring Lentivirus Vector Stocks for Replication-Competent Viruses
    • Panel: Introducing Genes into Mammalian Cells: Viral Vectors1209
    • Panel: Factors to Consider When Choosing a Viral Vector1211
    • Panel: The Major Types of Viruses Currently Used as Vectors1212
    • Panel: In Vivo Expression1221
    • Panel: Adenovirus Vectors1221
    • Panel: Adeno-Associated Virus Vectors1224
    • Panel: Retrovirus and Lentivirus Vectors1227
    • Panel: Additional Protocol: Preparation of a DNA Standard for qPCR1262
    • Panel: Adenovirus Vectors1322
    • Panel: AAV Vectors1323
    • Panel: Lentivirus Vectors1324
    • Panel: Basic Elements in Viral Vectors1326
    • Panel: Assays Done in Transduced Cells1328
    • Panel: Transgene Expression Cassettes1330
• Volume 3
  • Chapter 17: Analysis of Gene Regulation Using Reporter Systems1335
    • Protocol 1: Assay for -Galactosidase in Extracts of Mammalian Cells
    • Protocol 2: Single Luciferase Reporter Assay
    • Protocol 3: Dual Luciferase Reporter Assay
    • Protocol 4: Using ELISA to Measure GFP Production
    • Protocol 5: Generation of Cell Lines with Tetracycline-Regulated Gene Expression
    • Panel: Analysis of Gene Regulation Using Reporter Systems1335
    • Panel: Introduction to Reporter Systems1336
    • Panel: Reporter Genes Used in the Analysis of Regulatory Elements1336
    • Panel: Assaying for -Galactosidase in Extracts of Mammalian Cells1338
    • Panel: Assaying for Luciferase in Extracts of Mammalian Cells1339
    • Panel: Tetracycline-Responsive Expression Systems1341
    • Panel: Additional Protocol: Chemiluminescent Assay for -Galactosidase Activity1350
    • Panel: Additional Protocol: Selecting Stable Clones via Limiting Dilution of Suspension Cells1378
    • Panel: Fluorescent Proteins1381
    • Panel: Epitope Tagging1394
    • Panel: -Galactosidase1401
    • Panel: Luciferase1406
    • Panel: Tetracycline1409
  • Chapter 18: RNA Interference and Small RNA Analysis1415
    • Protocol 1: Preparation of siRNA Duplexes
    • Protocol 2: RNAi in Mammalian Cells by siRNA Duplex Transfection
    • Protocol 3: RNAi in Drosophila S2 Cells by siRNA Duplex Transfection
    • Protocol 4: Preparation of dsRNAs by In Vitro Transcription
    • Protocol 5: RNAi in Drosophila S2 Cells by dsRNA Soaking
    • Protocol 6: RNAi in Drosophila S2 Cells by dsRNA Transfection
    • Protocol 7: Analysis of Small RNAs by Northern Hybridization
    • Protocol 8: Analysis of Small RNAs by Quantitative Reverse Transcription PCR
    • Protocol 9: Construction of Small RNA Libraries for High-Throughput Sequencing
    • Protocol 10: Preparation of Antisense Oligonucleotides to Inhibit miRNA Function
    • Protocol 11: Inhibiting miRNA Function by Antisense Oligonucleotides in Cultured Mammalian Cells
    • Protocol 12: Inhibiting miRNA Function by Antisense Oligonucleotides in Drosophila S2 Cells
    • Panel: RNA Interference and Small RNA Analysis1415
    • Panel: Reverse Genetics by RNAi1419
    • Panel: Analysis of Small RNAs1425
    • Panel: Genome-Wide RNA Interference: Functional Genomics in the Postgenomics Era1472
    • Panel: StarFire Probes1478
  • Chapter 19: Expressing Cloned Genes for Protein Production, Purification, and Analysis1481
    • Protocol 1: Expression of Cloned Genes in E. coli Using IPTG-Inducible Promoters
    • Protocol 2: Expression of Cloned Genes Using the Baculovirus Expression System
    • Protocol 3: Expression of Cloned Genes in P. pastoris Using the Methanol-Inducible Promoter AOX1
    • Protocol 4: Preparation of Cell Extract for Purification of Soluble Proteins Expressed in E. coli
    • Protocol 5: Purification of Polyhistidine-Tagged Proteins by Immobilized Metal Affinity Chromatography
    • Protocol 6: Purification of Fusion Proteins by Affinity Chromatography on Glutathione Resin
    • Protocol 7: Solubilization of Expressed Proteins from Inclusion Bodies
    • Protocol 8: SDS-PAGE of Proteins
    • Protocol 9: Analysis of Proteins by Immunoblotting
    • Protocol 10: Methods for Measuring the Concentrations of Proteins
    • Panel: Expressing Cloned Genes for Protein Production, Purification, and Analysis1481
    • Panel: Choosing an Expression System1483
    • Panel: Choosing an Appropriate Expression Vector1488
    • Panel: Fusion Proteins1499
    • Panel: Optimization of Expression of Foreign Proteins1503
    • Panel: Additional Protocol: Small-Scale Test for Soluble Target Protein Expression1514
    • Panel: Alternative Protocol: Expression of Cloned Genes in E. coli Using the Arabinose BAD Promoter1520
    • Panel: Alternative Protocol: Subcellular Localization of Signal Peptide Fusion Proteins1522
    • Panel: Additional Protocol: Plaque Assay to Determine the Titer of the Baculovirus Stock1535
    • Panel: Alternative Protocol: Production of Bacmid DNA for Transfection into Insect Cells1538
    • Panel: Additional Protocol: Cryostorage of Yeast Cultures1553
    • Panel: Additional Protocol: Lysis of Yeast Cells Using Glass Beads1564
    • Panel: Alternative Protocol: Preparation of E. coil Cell Extract Using Gentle, Heat-Induced Enzymatic Lysis1566
    • Panel: Alternative Protocol: Preparation of E. coli Cell Extract Using FreezeThaw with Enzymatic Lysis by Lysozyme1568
    • Panel: Additional Protocol: Regenerating and Cleaning the Ni²NTA Resin1579
    • Panel: Alternative Protocol: Fast Performance Liquid Chromatography Purification of Histidine-Tagged Proteins1581
    • Panel: Alternative Protocol: Variations of Staining SDSPolyacrylamide Gels with Coomassie Brilliant Blue1609
    • Panel: Alternative Protocol: Staining SDSPolyacrylamide Gels with Silver Salts1611
    • Panel: Considerations for Membrane Protein Purification1632
    • Panel: Historical Footnote: Coomassie Brilliant Blue1636
  • Chapter 20: Cross-Linking Technologies for Analysis of Chromatin Structure and Function1637
    • Protocol 1: Formaldehyde Cross-Linking
    • Protocol 2: Preparation of Cross-Linked Chromatin for ChIP
    • Protocol 3: ChIP
    • Protocol 4: ChIPQuantitative PCR (ChIP-qPCR)
    • Protocol 5: ChIP-chip
    • Protocol 6: ChIP-seq
    • Protocol 7: Generation of 3C Libraries from Cross-Linked Cells
    • Protocol 8: Generation of ChIP-loop Libraries
    • Protocol 9: Generation of Control Ligation Product Libraries
    • Protocol 10: PCR Detection of 3C Ligation Products Present in 3C, ChIP-loop, and Control Libraries: Library Titration and Interaction Frequency Analysis
    • Protocol 11: 4C Analysis of 3C, ChIP-loop, and Control Libraries
    • Protocol 12: 5C Analysis of 3C, ChIP-loop, and Control Libraries
    • Panel: Cross-Linking Technologies for Analysis of Chromatin Structure and Function1637
    • Panel: Formaldehyde Cross-Linking to Interrogate Genomic Interactions1638
    • Panel: ChIP Analysis of ProteinDNA Interactions1638
    • Panel: 3C-Based Chromatin Interaction Analyses1641
    • Panel: Formaldehyde1701
    • Panel: What Is Captured by 3C-Based Assays?1702
  • Chapter 21: Mapping of In Vivo RNA-Binding Sites by UV-Cross-Linking Immunoprecipitation (CLIP)1703
    • Protocol 1: Optimization of Immunoprecipitation Stringency for CLIP
    • Protocol 2: UV Cross-Linking of Live Cells and Lysate Preparation
    • Protocol 3: RNase Titration, Immunoprecipitation, and SDS-PAGE
    • Protocol 4: 3-Linker Ligation and Size Selection by SDS-PAGE
    • Protocol 5: Isolation of the RNA Tags, 5-Linker Ligation, and Reverse Transcription PCR Amplification
    • Protocol 6: Sequencing of RNA CLIP Tags
    • Protocol 7: Gel Purification and Storage of RNA Linkers
    • Panel: Mapping of In Vivo RNA-Binding Sites by UV-Cross-Linking Immunoprecipitation (CLIP)1703
    • Panel: The Cross-Linking Immunoprecipitation Method1706
    • Panel: High-Throughput Sequencing (HITS) CLIP1708
    • Panel: Validation of CLIP Results1708
    • Panel: CLIP Method Variations1709
    • Panel: General Considerations in Planning CLIP Experiments1710
    • Panel: Alternative Protocol: 5-End Labeling of Dephosphorylated RL3 Linker1738
    • Panel: Mechanism and Specificity of UV-Protein Cross-Linking1756
    • Panel: HITS-CLIP Data Analysis1758
  • Chapter 22: Gateway-Compatible Yeast One-Hybrid and Two-Hybrid Assays1761
    • Protocol 1: Generating Yeast One-Hybrid DNA-Bait Strains
    • Protocol 2: Generating Yeast Two-Hybrid Bait Strains
    • Protocol 3: Identifying Interactors from an Activation Domain Prey Library
    • Protocol 4: High-Efficiency Yeast Transformation
    • Protocol 5: Colony Lift Colorimetric Assay for -Galactosidase Activity
    • Protocol 6: Yeast Colony PCR
    • Panel: Gateway-Compatible Yeast One-Hybrid and Two-Hybrid Assays1761
    • Panel: The Yeast Two-Hybrid (Y2H) System: Concept and Methodology1763
    • Panel: The Yeast One-Hybrid (Y1H) System: Concept and Methodology1767
    • Panel: Y2H and Y1H Assays: Advantages and Disadvantages1768
    • Panel: False Positives1769
    • Panel: Protocols for Yeast One-Hybrid and Two-Hybrid Systems1770
    • Panel: Alternative Protocol: Creating Entry Clones from DNA-Baits Generated by Annealing Primers1782
    • Panel: Why Integrate DNA-Baits?1808
    • Panel: Choosing a Vector and a Yeast Strain1809
    • Panel: Replica-Plating and Replica-Cleaning Using Velvets1810
    • Panel: Reagents and Buffers1811
    • Panel: Tris Buffers1828
    • Panel: Good Buffers1829
    • Panel: Phosphate Buffers (Gomori Buffers)1830
    • Panel: Phenol1834
    • Panel: Equilibration of Phenol1834
    • Panel: Phenol:Chloroform:Isoamyl Alcohol (25:24:1)1834
    • Panel: Deionization of Formamide1834
    • Panel: Blocking Agents Used for Nucleic Acid Hybridization1836
    • Panel: Blocking Agents Used for Western Blotting1836
    • Panel: Commonly Used Techniques1843
    • Panel: Siliconizing Glassware, Plasticware, and Glass Wool1843
    • Panel: Preparation of RNase-Free Glassware1844
    • Panel: Hemocytometry Counting1846
    • Panel: Viability Staining1847
    • Panel: Precipitation of Nucleic Acids with Trichloroacetic Acid1849
    • Panel: Removing Ethidium Bromide from DNA1851
    • Panel: Disposing of Ethidium Bromide1851
    • Panel: Decontamination of Concentrated Solutions of Ethidium Bromide (Solutions Containing >0.5 mg/mL)1851
    • Panel: Decontamination of Dilute Solutions of Ethidium Bromide (e.g., Electrophoresis Buffer Containing 0.5 g/mL Ethidium Bromide)1852
    • Panel: Commercial Decontamination Kits1852
    • Panel: Detection Systems1855
    • Panel: Ethidium Bromide1855
    • Panel: Methylene Blue1857
    • Panel: SYBR Dyes1857
    • Panel: Chemiluminescent Labels1860
    • Panel: Chemiluminescent Enzyme Assays1861
    • Panel: Commercial Reagents, Kits, and Luminometers1863
    • Panel: Horseradish Peroxidase1865
    • Panel: Digoxygenin1869
    • Panel: BCIP1873
    • Panel: AMPPD1876
    • Panel: Immunoglobulin-Binding Proteins: Proteins A, G, and L1879
    • Panel: General Safety and Hazardous Material1885

Separation of RNA according to Size: Electrophoresis of RNA through Denaturing Urea Polyacrylamide Gels

(Protocol summary only for purposes of this preview site)

Thin (0.41.5 mm) polyacrylamide-urea gels provide high resolution of RNAs up to 1000 nucleotides in size and are capable of resolving single-stranded fragments of RNA that differ in length by as little as 1 nucleotide. Polyacrylamide gels are chemically cross-linked by the polymerization of acrylamide with a cross-linking agent, usually N,N-methylene bisacrylamide. The polymerization initiates by free radical formation usually carried out using ammonium persulfate as the initiator and N,N,N,N-tetramethylene diamine (TEMED) as the catalyst (^{Chrambach and Rodbard 1972}). The presence of the denaturant urea in the gel prevents the formation of secondary structure and ensures that the RNA molecules migrate through the gel as linear species.



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