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Control of dinucleoside polyphosphates by the FHIT-homologous HNT2 gene, adenine biosynthesis and heat shock in Saccharomyces cerevisiae

机译:FHIT同源HNT2基因对酿酒酵母中二核苷多磷酸的控制,酿酒酵母中的腺嘌呤生物合成和热休克

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摘要

Background: The FHIT gene is lost early in the development of many tumors. Fhit possesses intrinsic ApppA hydrolase activity though ApppA cleavage is not required for tumor suppression. Because a mutant form of Fhit that is functional in tumor suppression and defective in catalysis binds ApppA well, it was hypothesized that Fhit-substrate complexes are the active, signaling form of Fhit. Which substrates are most important for Fhit signaling remain unknown. Results: Here we demonstrate that dinucleoside polyphosphate levels increase 500-fold to hundreds of micromolar in strains devoid of the Saccharomyces cerevisiae homolog of Fhit, Hnt2. Accumulation of dinucleoside polyphosphates is reversed by re-expression of Hnt2 and is active site-dependent. Dinucleoside polyphosphate levels depend on an intact adenine biosynthetic pathway and time in liquid culture, and are induced by heat shock to greater than 0.1 millimolar even in Hnt2+ cells. Conclusions: The data indicate that Hnt2 hydrolyzes both ApppN and AppppN in vivo and that, in heat-shocked, adenine prototrophic yeast strains, dinucleoside polyphosphates accumulate to levels in which they may saturate Hnt2.
机译:背景:FHIT基因在许多肿瘤的发生早期就丢失了。 Fhit具有内在的ApppA水解酶活性,尽管抑制肿瘤不需要ApppA裂解。因为Fhit的突变体形式具有抑制肿瘤的功能并且催化缺陷,因此它与ApppA结合良好,因此可以假设Fhit-底物复合物是Fhit的活性信号形式。哪些底物对Fhit信号最重要,仍然未知。结果:在这里,我们证明了在没有Fhit,Hnt2啤酒酵母同源物的菌株中,二核苷多磷酸酯水平增加了500倍,达到数百微摩尔。 Hnt2的重新表达可以逆转聚磷酸二核苷的积累,并且是活性位点依赖性的。二核苷多磷酸酯水平取决于液体培养中完整的腺嘌呤生物合成途径和时间,并且即使在Hnt2 +细胞中,也会因热激而诱导大于0.1毫摩尔。结论:数据表明,Hnt2在体内水解ApppN和AppppN,并且在热激的腺嘌呤原养型酵母菌株中,二核苷多磷酸盐积累到可以使Hnt2饱和的水平。

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