渗透调节TAQ聚合酶基因在大肠杆菌中的表达。

Yeosvany Cabrera Artiles, Duniesky Martínez García, Enrique R Pérez Cruz, Gabriel J Márquez Perera, Manuel Luis Feble
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引用次数: 0

摘要

在渗透诱导启动子proU的作用下,将水热菌DNA聚合酶I (Taq Pol I)基因克隆到pOSEX4质粒中,并在大肠杆菌MKH13中表达。该酶在聚合酶试验中的适用性通过标准35S dATP掺入试验和PCR确定。在生长介质渗透压控制下,分析了该体系在不同培养基和不同氯化钠浓度下Taq Pol I的表达情况。渗透压对菌株生长和Taq Pol I表达的影响表明,氯化钠浓度的增加限制了菌株的生长。NaCl浓度为0.25 M时活性最大;在较高的渗透压值下,我们发现活性出乎意料地下降。这是首次使用pOSEX载体表达异源蛋白的报道,在仅使用NaCl或其他不渗透渗透物的生物技术过程中,它具有调节、无毒、简单和经济的优势。
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Osmoregulated TAQ polymerase gene expression in Escherichia coli.

The Thermus aquaticus DNA Polymerase I (Taq Pol I) gene was cloned into the pOSEX4 plasmid under the osmo-inducible promoter proU and subsequently expressed into the Escherichia coli MKH13 strain. The suitability of the enzyme in polymerase assays was determined in standard 35S dATP incorporation tests and by PCR. The Taq Pol I expression in this system, which is under the control of the osmotic pressure in the growth medium, was analyzed in different media and in different sodium chloride concentrations. A study of the osmolarity effects in the growth of the strain and in Taq Pol I expression shows that an increase in sodium chloride concentration limits the growth. At 0.25 M of NaCl maximum activity was observed; at higher values of osmolarity, we found an unexpected decline of activity. This is the first report of using the pOSEX vector for the expression of an heterologous protein and it is very advantageous to make a regulated, non toxic, simple and cost-effective manner of induction in a biotechnology process using just NaCl or other non-permeable osmolyte.

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