Literature DB >> 20147122

Optimization and troubleshooting in PCR.

Kenneth H Roux.   

Abstract

The use of polymerase chain reaction (PCR) to generate large amounts of a desired product can be a double-edged sword. Failure to amplify under optimum conditions can lead to the generation of multiple undefined and unwanted products, even to the exclusion of the desired product. At the other extreme, no product may be produced. A typical response at this point is to vary one or more of the many parameters that are known to contribute to primer-template fidelity and primer extension. High on the list of optimization variables are Mg(++) concentrations, buffer pH, and cycling conditions. With regard to the last, the annealing temperature is most important. The situation is further complicated by the fact that some of the variables are quite interdependent. For example, because dNTPs directly chelate a proportional number of Mg(++) ions, an increase in the concentration of dNTPs decreases the concentration of free Mg(++) available to influence polymerase function. This article discusses various optimization strategies, including touchdown PCR and hot-start PCR.

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Year:  2009        PMID: 20147122     DOI: 10.1101/pdb.ip66

Source DB:  PubMed          Journal:  Cold Spring Harb Protoc        ISSN: 1559-6095


  23 in total

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5.  Combining Structure-Function and Single-Molecule Studies on Cytoplasmic Dynein.

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Review 6.  Design of Experiments As a Tool for Optimization in Recombinant Protein Biotechnology: From Constructs to Crystals.

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8.  Optimization of PCR conditions for amplification of GC-Rich EGFR promoter sequence.

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9.  Robust Optimization of Biological Protocols.

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