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A pull-down procedure for the identification of unknown GEFs for small GTPases

机译:用于识别小型GTPases的未知GEF的下拉程序

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摘要

Members of the family of small GTPases regulate a variety of important cellular functions. In order to accomplish this, tight temporal and spatial regulation is absolutely necessary. The two most important factors for this regulation are GTPase activating proteins (GAPs) and guanine nucleotide exchange factors (GEFs), the latter being responsible for the activation of the GTPase downstream pathways at the correct location and time. Although a large number of exchange factors have been identified, it islikely that a similarly large number remains unidentified. We have therefore developed a procedure to specifically enrich GEF proteins from biological samples making use of the high affinity binding of GEFs to nucleotide-free GTPases. In order to verifythe results of these pull-down experiments, we have additionally developed two simple validation procedures: An in vitro transcription/translation system coupled with a GEF activity assay and a yeast two-hybrid screen for detection of GEFs. Although theprocedures were established and tested using the Rab protein Sec4, the similar basic principle of action of all nucleotide exchange factors will allow the method to be used for identification of unknown GEFs of small GTPases in general.
机译:小GTP酶家族的成员调节多种重要的细胞功能。为此,绝对需要严格的时间和空间调节。该调节的两个最重要因素是GTPase激活蛋白(GAP)和鸟嘌呤核苷酸交换因子(GEF),后者负责在正确的位置和时间激活GTPase下游途径。尽管已识别出许多交换因子,但很可能仍未识别出同样大量的交换因子。因此,我们开发了一种程序,可以利用GEF与不含核苷酸的GTPases的高亲和力结合,从生物样品中特异性富集GEF蛋白。为了验证这些下拉实验的结果,我们还开发了两种简单的验证程序:体外转录/翻译系统,结合GEF活性测定法和酵母双杂交筛选,用于检测GEF。尽管已使用Rab蛋白Sec4建立了程序并进行了测试,但所有核苷酸交换因子的相似基本作用原理将使该方法通常可用于鉴定小GTP酶的未知GEF。

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