BioOne.org will be down briefly for maintenance on 17 December 2024 between 18:00-22:00 Pacific Time US. We apologize for any inconvenience.
How to translate text using browser tools
1 May 2007 Making Taq DNA polymerase in the undergraduate biology laboratory
Philip Ferralli, John Duick Egan, Floyd Lester Erickson
Author Affiliations +
Abstract

The polymerase chain reaction (PCR) is an important technique for biology students to learn. PCR utilizes DNA polymerases isolated from archaea or bacteria, like Thermus aquaticus (Taq), to amplify target DNA sequences. In this paper we describe lab activities where students clone the gene for, express, and purify Taq DNA polymerase and assay for its activity. These lab activities employ plasmids containing multiple components of the lac operon thereby giving students practical experience with a genetic regulatory system they learn about in the classroom. Taq DNA polymerase purification simply involves cell lysis, a heat incubation step, and centrifugation, with the resulting supernatant containing highly pure and active Taq DNA polymerase.

Philip Ferralli, John Duick Egan, and Floyd Lester Erickson "Making Taq DNA polymerase in the undergraduate biology laboratory," BIOS 78(2), 69-74, (1 May 2007). https://doi.org/10.1893/0005-3155(2007)78[69:MTDPIT]2.0.CO;2
Received: 8 September 2006; Accepted: 1 February 2007; Published: 1 May 2007
RIGHTS & PERMISSIONS
Get copyright permission
Back to Top