首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Two Drosophila melanogaster mutations block successive steps of de novo purine synthesis.
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Two Drosophila melanogaster mutations block successive steps of de novo purine synthesis.

机译:两个果蝇黑变种突变阻止了从头嘌呤合成的连续步骤。

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摘要

Drosophila melanogaster purine auxotrophs ade2(1) and ade3(1) have been characterized biochemically. The ade2(1) strain is deficient in the fourth step of the de novo purine synthetic pathway catalyzed by phosphoribosylglycinamidine synthase (phosphoribosylformylglycinamide amidotransferase). The ade3(1) strain is deficient in the previous step catalyzed by phosphoribosylglycinamide formyltransferase (GART). The mutation responsible for the slightly leaky ade3(1) phenotype was characterized further. First, the mutant GART polypeptide was found to be of normal size and present at normal levels. Second, the GART-encoding region of the mutant was cloned, inserted into a yeast-Escherichia coli shuttle vector, and used to transform mutant yeast. Transformants showed very slight in vivo activity when compared to wild type, verifying that the mutation is in the GART coding sequence. Lastly, the region of the gene encoding GART activity from mutant and inbred parental strain flies was completely sequenced. A single base transition was found, leading to the substitution of a serine for a highly conserved glycine. These two mutations provide examples of blocks in the de novo purine synthetic pathway in a whole animal.
机译:果蝇黑色素嘌呤营养缺陷型ade2(1)和ade3(1)已被生化表征。 ade2(1)菌株在由磷酸核糖基甘氨酰胺合酶(磷酸核糖基甲酰基甘氨酰胺酰胺转移酶)催化的嘌呤从头合成途径的第四步中缺乏作用。 ade3(1)菌株在以前的步骤中由磷酸核糖基甘氨酰胺甲酰转移酶(GART)催化。负责轻微泄漏的ade3(1)表型的突变被进一步表征。首先,发现突变体GART多肽具有正常大小并且以正常水平存在。第二,克隆突变体的GART编码区,将其插入酵母-大肠杆菌穿梭载体中,并用于转化突变酵母。与野生型相比,转化子显示出非常轻微的体内活性,证实了该突变位于GART编码序列中。最后,对来自突变和近交亲本菌株蝇的GART活性编码基因的区域进行了完整测序。发现单个碱基的转变,导致丝氨酸被高度保守的甘氨酸取代。这两个突变提供了整个动物中从头嘌呤合成途径中的嵌段实例。

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