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A unified approach towards Trypanosoma brucei functional genomics using Gibson assembly

机译:使用Gibson组装对锥蛋白酶瘤葡萄球菌瘤功能基因组学的统一方法

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Trypanosoma brucei is the causative agent of human African trypanosomiasis and nagana in cattle. Recent advances in high throughput phenotypic and interaction screens have identified a wealth of novel candidate proteins for diverse functions such as drug resistance, life cycle progression, and cytoskeletal biogenesis. Characterization of these proteins will allow a more mechanistic understanding of the biology of this important pathogen and could identify novel drug targets. However, methods for rapidly validating and prioritizing these potential targets are still being developed. While gene tagging via homologous recombination and RNA interference are available in T. brucei, a general strategy for creating the most effective constructs for these approaches is lacking. Here, we adapt Gibson assembly, a one-step isothermal process that rapidly assembles multiple DNA segments in a single reaction, to create endogenous tagging, overexpression, and long hairpin RNAi constructs that are compatible with well-established T. brucei vectors. The generality of the Gibson approach has several advantages over current methodologies and substantially increases the speed and ease with which these constructs can be assembled. (C) 2016 Elsevier B.V. All rights reserved.
机译:葡萄球菌瘤Brucei是人类非洲锥虫病的致病剂和牛的纳卡纳。高吞吐量表型和相互作用屏幕的最新进展已经确定了一种丰富的新候选蛋白,用于不同的功能,例如耐药性,生命周期进展和细胞骨骼生物发生。这些蛋白质的表征将使对这种重要病原体的生物学进行更具机制的理解,并且可以识别新型药物靶标。然而,仍在开发出快速验证和优先考虑这些潜在目标的方法。虽然通过同源重组和RNA干扰的基因标记可在T. Brucei中获得,但缺乏为这些方法产生最有效构建的一般策略。在这里,我们适应Gibson组装,一种一步等温处理,即在单一反应中快速组装多个DNA段,以产生与成熟的T.Brucei载体相容的内源性标记,过表达和长发夹rnai构建体。 Gibson方法的一般性与电流方法相比具有若干优点,并且基本上增加了这些构造的速度和易于组装的速度。 (c)2016年Elsevier B.v.保留所有权利。

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