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黑腹果蝇和拟果蝇中α-淀粉酶基因位点的结构组织。

Structural organization of the alpha-amylase gene locus in Drosophila melanogaster and Drosophila miranda.

作者信息

Doane W W, Gemmill R M, Schwartz P E, Hawley S A, Norman R A

出版信息

Isozymes Curr Top Biol Med Res. 1987;14:229-66.

PMID:3110097
Abstract

Chromosomal sites belonging to the alpha-amylase gene family have been identified in D. melanogaster and D. miranda and in the sibling species of miranda, pseudoobscura, and persimilis. Two sites occur in chromosome 2 of melanogaster; one contains the Amy gene locus (54A) and the other an amylase "pseudogene" (53CD). Two sites of homology exist at 73A and 78C and perhaps another at 81BC in chromosome 3 of pseudoobscura and persimilis and in the homologous regions of the X2 chromosome in miranda. The active Amy locus is apparently at 73A. The structural organization of cloned sequences from this multigene family in melanogaster and miranda is under analysis, with emphasis on the functional Amy gene region. Electrophoretic variants of amylase have served as invaluable tools in these studies. For melanogaster, their use as genetic markers enabled us to positively identify our lambda Dm65 clone of the Amy locus and to show that it contains two functional copies of the structural gene for alpha-amylase. Amylase isozymes are now being used in P element-mediated transformation experiments aimed at defining regulatory elements for the temporal and spatial control of amylase expression during development and in response to dietary glucose. In miranda, electrophoretic variants of amylase were useful in assigning the Amy locus to chromosome X2, and they continue to serve as essential markers in our study of the evolution of dosage compensation for amylase expression in males of this species. Restriction maps of the Amy locus in 7 strains of D. melanogaster indicate that despite the worldwide origins of the chromosome samples, all contain a duplication of the amylase structural gene at this locus regardless of whether they produce two alpha-amylase isozymes, a single variant, or none. We have aligned these maps with the genetic and cytological maps of chromosome 2R in melanogaster and assigned alleles for different amylase isozymes to either the proximal or distal Amy gene copy in a number of strains. Restriction site polymorphism is relatively limited at the Amy locus, but some strain-specific rearrangements exist. The locus of two strains with reduced amylase activity, Amy1 (CA 1) and Amy "null", contain anomalies--an insertion in the former and an inversion in the latter. Causal relationships are being sought between the level of amylase expression in these strains and the position of their respective anomalies.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

在黑腹果蝇、拟暗果蝇以及拟暗果蝇的近缘种米兰达果蝇、伪暗果蝇和佩氏果蝇中,已鉴定出属于α -淀粉酶基因家族的染色体位点。在黑腹果蝇的2号染色体上有两个位点;一个含有Amy基因座(54A),另一个含有一个淀粉酶“假基因”(53CD)。在伪暗果蝇和佩氏果蝇的3号染色体以及米兰达果蝇X2染色体的同源区域中,在73A和78C处存在两个同源位点,在81BC处可能还有另一个同源位点。活性Amy基因座显然在73A处。目前正在分析黑腹果蝇和米兰达果蝇中这个多基因家族克隆序列的结构组织,重点是功能性Amy基因区域。淀粉酶的电泳变体在这些研究中是非常有价值的工具。对于黑腹果蝇,将其用作遗传标记使我们能够明确鉴定出Amy基因座的λDm65克隆,并表明它包含α -淀粉酶结构基因的两个功能拷贝。淀粉酶同工酶目前正用于P因子介导的转化实验,旨在确定在发育过程中以及对饮食葡萄糖作出反应时淀粉酶表达的时空控制的调控元件。在米兰达果蝇中,淀粉酶的电泳变体有助于将Amy基因座定位到X2染色体上,并且它们在我们对该物种雄性淀粉酶表达剂量补偿进化的研究中仍然是重要的标记。对7个黑腹果蝇品系中Amy基因座的限制性图谱分析表明,尽管染色体样本来自世界各地,但无论它们产生两种α -淀粉酶同工酶、一种变体还是不产生变体,该基因座都包含淀粉酶结构基因的重复。我们已将这些图谱与黑腹果蝇2R染色体的遗传图谱和细胞学图谱进行比对,并在一些品系中为不同的淀粉酶同工酶等位基因指定了近端或远端Amy基因拷贝。在Amy基因座处,限制性位点多态性相对有限,但存在一些品系特异性的重排。两个淀粉酶活性降低的品系,Amy1(CA 1)和Amy“无效”,其基因座存在异常——前者有一个插入,后者有一个倒位。正在寻找这些品系中淀粉酶表达水平与其各自异常位置之间的因果关系。(摘要截短至400字)

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