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PCR Cloning Protocols

From Molecular Cloning to Genetic Engineering

  • Book
  • © 1997

Overview

Editors:
  1. Bruce A. White

    1. Department of Anatomy, University of Connecticut Health Center, Farmington

    View editor publications

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Part of the book series: Methods in Molecular Biology (MIMB, volume 67)

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Table of contents (44 protocols)

  1. Front Matter

    Pages i-xiv
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  2. Performing and Optimizing PCR

    1. Front Matter

      Pages 1-1
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    2. PCR

      • Lori A. Kolmodin, J. Fenton Williams
      Pages 3-15

    3. XL PCR Amplification of Long Targets From Genomic DNA

      • Suzanne Cheng, Lori A. Kolmodin
      Pages 17-29

    4. Amplification of DNA Sequences Up To 5 kb from Small Amounts of Genomic DNA Using Tub DNA Polymerase

      • Helen B. Forrester, Ian R. Radford
      Pages 31-38

    5. One-Step Optimization Using Touchdown and Stepdown PCR

      • Kenneth H. Roux, Karl H. Hecker
      Pages 39-45

    6. GC-Rich Template Amplification by Inverse PCR

      • Alain Moreau, Colette Duez, Jean Dusart
      Pages 47-53

    7. Coupled One-Step Reverse Transcription and Polymerase Chain Reaction Procedure for Cloning Large cDNA Fragments

      • Jyrki T. Aatsinki
      Pages 55-60

  3. Cloning PCR Products

    1. Front Matter

      Pages 61-61
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    2. Using T4 DNA Polymerase to Generate Clonable PCR Products

      • Kai Wang
      Pages 63-68

    3. Rapid (Ligase-Free) Subcloning of PCR Products

      • Alan R. Shuldiner, Keith Tanner
      Pages 69-78

    4. Cloning PCR Products Utilizing the T/A Overhang and a Kit

      • Melissa Lail-Trecker
      Pages 79-88

    5. Cloning Unmodified PCR Products Using Engineered Xcml Restriction Sites in a Portable Cassette

      • Alessandro Testori, Paul Sollitti
      Pages 89-100

    6. A T-Linker Strategy for Modification and Directional Cloning of PCR Products

      • Robert M. Horton, Raghavanpillai Raju, Bianca M. Conti-Fine
      Pages 101-110

    7. Recovery of DNA Amplification Products from Silver-Stained Polyacrylamide Gels

      • Gustavo Caetano-Anollés, Robert N. Trigiano
      Pages 111-127

  4. Mutagenesis, Recombination, and In Vitro Selection

    1. Front Matter

      Pages 129-129
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    2. Recombination and Site-Directed Mutagenesis Using Recombination PCR

      • Douglas H. Jones, Stanley C. Winistorfer
      Pages 131-140

    3. In Vitro Recombination and Mutagenesis of DNA

      • Robert M. Horton
      Pages 141-150

    4. In-Frame Cloning of Synthetic Genes Using PCR Inserts

      • James C. Pierce
      Pages 151-165

    5. Creation of Chimeric Junctions, Deletions, and Insertions by PCR

      • Geneviève Pont-Kingdon
      Pages 167-172
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About this book

The advent of PCR, with its power to amplify tiny amounts of DNA, quickly spawned the development of many analytical procedures that are widely used for detection, measurement, and characterization. However, creative investigators soon discovered the power of PCR for synthetic or preparative uses. This volume focuses on such preparative PCR protocols, which can be used in the cloning and modification of DNA. PCR Cloning Protocols: From Molecular Cloning to Genetic Engineer­ ing is divided into seven parts, each containing a collection of chapters address­ ing a general approach or goal. Part I presents basic PCR protocols, emphasizing optimizing conditions for (he amplification of DNA fragments of several kilobases in length. Part 11 offers several procedures for cloning PCR prod­ ucts, depending on whether a specific restriction site can be used in the clon­ ing vector, the PCR product is to be gel purified before cloning, or the fragmeni needs to be inserted in one or both orientations. Part III includes several pro­ tocols involved in the mutagenesis of DNA, either site-directed or not, as well as several approaches to recombinant PCR, either for mutagenesis or building a custom gene, as well as one chapter describing a specific use of in vitro selection. Part IV addresses the frequent need to amplify and clone segments of DNA that are to the right, left, or scattered within a stretch of DNA (either vector, chromosomal, or cDNA) of known sequence.

Reviews

This volume provides protocols useful to both the inexperienced and the experienced investigator. Most importantly it highlights the emerging role of PCR as a versatile tool for the molecular biologist eliminating many laborious and expensive techniques associated with traditional gene isolation and analysis.-Biochemical Education

Editors and Affiliations

  • Department of Anatomy, University of Connecticut Health Center, Farmington

    Bruce A. White

Bibliographic Information

  • Book Title: PCR Cloning Protocols

  • Book Subtitle: From Molecular Cloning to Genetic Engineering

  • Editors: Bruce A. White

  • Series Title: Methods in Molecular Biology

  • DOI: https://doi.org/10.1385/0896034836

  • Publisher: Humana Totowa, NJ

  • eBook Packages: Springer Protocols

  • Copyright Information: Humana Press 1997

  • eBook ISBN: 978-1-59259-553-2Published: 02 February 2008

  • Series ISSN: 1064-3745

  • Series E-ISSN: 1940-6029

  • Edition Number: 1

  • Number of Pages: XIV, 490

  • Topics: Biochemistry, general

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