Reevaluating the Capability of Taq DNA Polymerase: Long PCR Amplification

Hayan Lee; Kyung-Nam Kim; YK Chae

doi:10.2174/092986607780363934

ISSN: 0929-8665
E-ISSN: 1875-5305

Reevaluating the Capability of Taq DNA Polymerase: Long PCR Amplification
Authors: Hayan Lee¹, Kyung-Nam Kim² and YK Chae³
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¹ Department of Chemistry and 2Recombinant Protein Expression Center (RPEC), Sejong University,98 Gunja-Dong, Gwangjin-Gu, Seoul, Korea, 143-747. ² Department of Chemistry and 2Recombinant Protein Expression Center (RPEC), Sejong University,98 Gunja-Dong, Gwangjin-Gu, Seoul, Korea, 143-747. ³ Department of Chemistry and 2Recombinant Protein Expression Center (RPEC), Sejong University,98 Gunja-Dong, Gwangjin-Gu, Seoul, Korea, 143-747.
Source: Protein and Peptide Letters, Volume 14, Issue 4, Apr 2007, p. 321 - 323
DOI: https://doi.org/10.2174/092986607780363934
- Available online: 01 Apr 2007

Abstract

We tested the ability of Taq DNA polymerase (Taq) to amplify long DNA fragments and showed that, if the conditions were set properly, Taq could successfully perform the “long PCR” up to 24 kb. The conditions include: (1) longer primers, (2) a 2-step cycling, and (3) a “long buffer.” We propose that the most important requirements are the survival rate of Taq at high temperatures and that of the primers against the 5' to 3' exonuclease activity of Taq.

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2007-04-01

2025-05-23

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Article Type: Research Article

Keyword(s): long amplicons; primers; reaction buffer; Taq DNA polymerase

Reevaluating the Capability of Taq DNA Polymerase: Long PCR Amplification

Abstract

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