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通过酵母突变体互补法从马铃薯中分离和鉴定两个编码ATP硫酸化酶的cDNA克隆。

Isolation and characterization of two cDNA clones encoding ATP-sulfurylases from potato by complementation of a yeast mutant.

作者信息

Klonus D, Höfgen R, Willmitzer L, Riesmeier J W

机构信息

Institut für Genbiologische Forschung Berlin GmbH, Germany.

出版信息

Plant J. 1994 Jul;6(1):105-12. doi: 10.1046/j.1365-313x.1994.6010105.x.

DOI:10.1046/j.1365-313x.1994.6010105.x
PMID:7920699
Abstract

Sulfur plays an important role in plants, being used for the biosynthesis of amino acids, sulfolipids and secondary metabolites. After uptake sulfate is activated and subsequently reduced to sulfide or serves as donor for sulfurylation reactions. The first step in the activation of sulfate in all cases studied so far is catalyzed by the enzyme ATP-sulfurylase (E.C. 2.7.7.4.) which catalyzes the formation of adenosine-5'-phosphosulfate (APS). Two cDNA clones from potato encoding ATP-sulfurylases were identified following transformation of a Saccharomyces cerevisiae mutant deficient in ATP-sulfurylase activity with a cDNA library from potato source leaf poly(A)+ RNA cloned in a yeast expression vector. Several transformants were able to grow on a medium with sulfate as the only sulfur source, this ability being strictly linked to the presence of two classes of cDNAs. The clones StMet3-1 and StMet3-2 were further analyzed. DNA analysis revealed an open reading frame encoding a protein with a molecular mass of 48 kDa in the case of StMet3-1 and 52 kDa for StMet3-2. The deduced polypeptides are 88% identical at the amino acid level. The clone StMet3-2 has a 48 amino acid N-terminal extension which shows common features of a chloroplast transit peptide. Sequence comparison of the ATP-sulfurylase Met3 from Saccharomyces cerevisiae with the cDNA StMet3-1 (StMet3-2) reveals 31% (30%) identity at the amino acid level. Protein extracts from the yeast mutant transformed with the clone StMet3-1 displayed ATP-sulfurylase activity. RNA blot analysis demonstrated the expression of both genes in potato leaves, root and stem, but not in tubers.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

硫在植物中起着重要作用,用于氨基酸、硫脂和次生代谢物的生物合成。吸收后,硫酸盐被激活,随后还原为硫化物或作为磺酰化反应的供体。在迄今为止研究的所有情况下,硫酸盐激活的第一步由ATP硫酸化酶(E.C. 2.7.7.4.)催化,该酶催化形成腺苷-5'-磷酸硫酸(APS)。在用酵母表达载体克隆的马铃薯源叶聚腺苷酸加尾RNA的cDNA文库转化缺乏ATP硫酸化酶活性的酿酒酵母突变体后,鉴定出两个来自马铃薯编码ATP硫酸化酶的cDNA克隆。几个转化体能够在以硫酸盐作为唯一硫源的培养基上生长,这种能力与两类cDNA的存在密切相关。对克隆StMet3-1和StMet3-2进行了进一步分析。DNA分析显示,在StMet3-1的情况下,有一个开放阅读框编码一个分子量为48 kDa的蛋白质,而StMet3-2编码的蛋白质分子量为52 kDa。推导的多肽在氨基酸水平上有88%的同一性。克隆StMet3-2有一个48个氨基酸的N端延伸,显示出叶绿体转运肽的共同特征。酿酒酵母的ATP硫酸化酶Met3与cDNA StMet3-1(StMet3-2)的序列比较显示,在氨基酸水平上有31%(30%)的同一性。用克隆StMet3-1转化的酵母突变体的蛋白质提取物显示出ATP硫酸化酶活性。RNA印迹分析表明这两个基因在马铃薯的叶、根和茎中表达,但在块茎中不表达。(摘要截短于250字)

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