A simple method for in-house Pfu DNA polymerase purification for high-fidelity PCR amplification

Prabu  Siva Sankar; Marimuthu  Citartan; Aminah  Ahmed Siti; Boris  V. Skryabin; Timofey  S. Rozhdestvensky; Goot  Heah Khor; Thean  Hock Tang

doi:10.18502/ijm.v11i2.1085

Prabu Siva Sankar
Marimuthu Citartan
Aminah Ahmed Siti
Boris V. Skryabin
Timofey S. Rozhdestvensky
Goot Heah Khor
Thean Hock Tang

DOI: https://doi.org/10.18502/ijm.v11i2.1085

Keywords: Protein expression; Pyrococcus furiosus; DNA polymerase; Polymerase chain reaction

Abstract

Background and Objectives: Pfu DNA polymerase is an enzyme that exhibits the lowest error rate in the 3´ to 5´ exonucle- ase (proofreading) activity during DNA synthesis in Polymerase Chain Reactions (PCRs). This study was aimed to express and purify Pfu DNA polymerase in a bacterial expression system under a simple purification method.

Materials and Methods: Pfu polymerase gene sequence, derived from Pyrocuccus furiosus (Pfu) genomic DNA, was cloned and overexpressed in E. coli BL21 (DE3) pLysS. Upon overexpression, bacterial lysate containing the Pfu DNA polymerase was heated at 94°C for 5 minutes. Pfu DNA polymerase having high thermal stability was retained while the other bacterial proteins were denatured. The resulting thermo stable Pfu DNA polymerase was separated from the other debris of the dena- tured proteins by simple centrifugation.

Results: The enzymatic activity of the resulting Pfu DNA polymerase was estimated by comparing with the commer- cial Pfu DNA Polymerases. An estimated 50000 units of functional Pfu DNA polymerase was produced from a 400 ml culture.

Conclusion: The in-house produced Pfu DNA Polymerase could be used for routine amplification that requires high-fidelity

such as cloning and DNA sequencing.