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Novel properties of recombinant Sso7d-Taq DNA polymerase purified using aqueous two-phase extraction: Utilities of the enzyme in viral diagnosis

机译:水相两相法纯化的重组Sso7d-Taq DNA聚合酶的新特性:该酶在病毒诊断中的实用性

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摘要

Using Sso7d from Sulfolobus solfataricus as the DNA binding protein fused to Taq DNA polymerase at its amino terminus, we report the hyper-expression and a novel purification methodology of Sso7d-Taq polymerase (S-Taq) using aqueous two-phase extraction system followed by Ni-affinity chromatography. The utility of such a fusion enzyme in carrying out PCR of human genes from whole blood directly and in detecting hepatitis B virus from clinical samples is demonstrated in this article. We present data on the enhanced thermo-stability of S-Taq DNA polymerase over Taq DNA polymerase and also provide evidence of its higher stability with detergents in comparison to Taq polymerase. The purified S-Taq protein showed acceptable limits of host genomic DNA levels without the use of DNases and other DNA precipitating agents and shows promising potential for use in PCR based diagnostics, in-situ PCR’s and forensic science.
机译:使用来自Sulfolobus solfataricus的Sso7d作为在Taq DNA聚合酶氨基端融合的DNA结合蛋白,我们报道了Sso7d-Taq聚合酶(S-Taq)的超表达和新型纯化方法,该方法使用水相两相萃取系统,然后镍亲和色谱。本文证明了这种融合酶在直接从全血中进行人类基因PCR以及从临床样本中检测乙型肝炎病毒方面的实用性。我们提供了有关Taq DNA聚合酶增强S-Taq DNA聚合酶热稳定性的数据,并且还提供了与Taq聚合酶相比,它与洗涤剂相比具有更高稳定性的证据。纯化的S-Taq蛋白在不使用DNase和其他DNA沉淀剂的情况下,显示出可接受的宿主基因组DNA水平极限,并显示出可用于基于PCR的诊断,原位PCR和法医学的潜力。

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