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Development of a defined medium for heterologous expression in Leishmania tarentolae.

机译:开发一种用于塔氏利什曼原虫中异源表达的确定培养基。

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摘要

A defined medium is essential for studying nutritional requirements of microorganisms and for selective supplementation of necessary substances. Hemin is an essential ingredient for growth of Leishmania tarentolae, but tends to precipitate in aqueous solutions without further stabilization. These aggregates disturb the measurement of the optical density or the cell density and the following downstream processing. Therefore, we were looking for stabilizing substances and established a PEG-hemin-solution, which avoided flocculation and allowed the cultivation of L. tarentolae in a medium, which we termed SFP(II) medium. With addition of RNA from Saccharomyces cerevisiae to SFP(II) medium the SFP(III) medium was established. In this medium, the specific cell division rate was increased (0.103 h(-1)) and stable for longer periods of time. The evaluation of the SFP(III) medium was done in shaker flasks by successful expression and segregation of the SAG2 protein, one of the main surface antigens of Toxoplasma gondii. With establishment and evaluation of this defined medium, the status of the Leishmania tarentolae expression system as an alternative to commonly used cell cultures is supported.
机译:确定的培养基对于研究微生物的营养需求和选择性补充必需物质至关重要。血红素是塔氏Leishmania tarentolae生长的必需成分,但趋于在水溶液中沉淀而不进一步稳定。这些聚集体干扰了光密度或细胞密度的测量以及随后的下游处理。因此,我们正在寻找稳定化的物质并建立了PEG-hemin溶液,该溶液可避免絮凝,并允许在一种称为SFP(II)的培养基中培养塔伦特氏杆菌。通过将来自酿酒酵母的RNA添加到SFP(II)培养基中,建立了SFP(III)培养基。在这种介质中,比细胞分裂率增加(0.103 h(-1)),并在更长的时间内保持稳定。通过成功表达和分离SAG2蛋白(弓形虫的主要表面抗原之一),在摇瓶中对SFP(III)培养基进行了评估。通过建立和评估这种确定的培养基,可以支持塔氏Leishmania tarentolae表达系统作为常用细胞培养的替代品。

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