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果蝇中的钼羟化酶。III. 低黄嘌呤脱氢酶基因的进一步特征分析。

Molybdenum hydroxylases in Drosophila. III. Further characterization of the low xanthine dehydrogenase gene.

作者信息

Schott D R, Baldwin M C, Finnerty V

出版信息

Biochem Genet. 1986 Aug;24(7-8):509-27. doi: 10.1007/BF00504332.

Abstract

The biochemical effects of several newly induced low xanthine dehydrogenase (lxd) mutations in Drosophila melanogaster were investigated. When homozygous, all lxd alleles simultaneously interrupt each of the molybdoenzyme activities to approximately the same levels: xanthine dehydrogenase, 25%; aldehyde oxidase, 12%; pyridoxal oxidase, 0%; and sulfite oxidase, 2% as compared to the wild type. In order to evaluate potentially small complementation or dosage effects, mutant stains were made coisogenic for 3R. These enzymes require a molybdenum cofactor, and lxd cofactor levels are also reduced to less than 10% of the wild type. These low levels of molybdoenzyme activities and cofactor activity are maintained throughout development from late larval to adult stages. The lxd alleles exhibit a dosage-dependent effect on molybdoenzyme activities, indicating that these mutants are leaky for wild-type function. In addition, cofactor activity is dependent upon the number of lxd+ genes present. The lxd mutation results in the production of more thermolabile XDH and AO enzyme activities, but this thermolability is not transferred with the cofactor to a reconstituted Neurospora molybdoenzyme. The lxd gene is localized to salivary region 68A4-9, 0.1 map unit distal to the superoxide dismutase (Sod) gene.

摘要

对果蝇中几个新诱导产生的低黄嘌呤脱氢酶(lxd)突变的生化效应进行了研究。当这些lxd等位基因纯合时,它们会同时将每种钼酶的活性阻断至大致相同的水平:与野生型相比,黄嘌呤脱氢酶为25%;醛氧化酶为12%;吡哆醛氧化酶为0%;亚硫酸盐氧化酶为2%。为了评估潜在的微小互补或剂量效应,使突变品系在3R区域同基因。这些酶需要钼辅因子,且lxd辅因子水平也降至野生型的不到10%。从幼虫后期到成虫阶段的整个发育过程中,这些低水平的钼酶活性和辅因子活性都得以维持。lxd等位基因对钼酶活性表现出剂量依赖性效应,这表明这些突变体对于野生型功能是渗漏的。此外,辅因子活性取决于所存在的lxd +基因的数量。lxd突变导致产生更多热不稳定的XDH和AO酶活性,但这种热不稳定性不会随辅因子转移至重组的粗糙脉孢菌钼酶。lxd基因定位于唾液腺区域68A4 - 9,在超氧化物歧化酶(Sod)基因远端0.1个图距处。

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