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黑腹果蝇梅干基因座的分离与特性分析。

Isolation and characterization of the prune locus of Drosophila melanogaster.

作者信息

Teng D H, Bender L B, Engele C M, Tsubota S, Venkatesh T

机构信息

Institute of Molecular Biology, University of Oregon, Eugene 97403.

出版信息

Genetics. 1991 Jun;128(2):373-80. doi: 10.1093/genetics/128.2.373.

Abstract

The complementary lethal interaction between the prune (pn) and Killer of prune loci of Drosophila melanogaster is an unusual and highly specific phenomenon. A lesion in pn results in a brownish-purple color of the compound eyes, while the conditional dominant Killer of prune mutation exhibits no phenotype by itself. However, a hemizygous or homozygous pn mutant carrying a copy of the Killer of prune gene dies during the late second to third instar stage of larval development. As a step toward understanding the molecular nature of this lethality and the role of pn in pigment biosynthesis, we have cloned the pn locus by using a transposon tag in the P element-induced allele, pn38. In addition, seven independent revertant lines were generated by the remobilization of transposons in pn38. The pn gene is located in a region that is transcriptionally active, and the isolated cDNAs that correspond to this area fall into three transcription units: I, II and III. Southern analysis shows that the restriction fragment length polymorphisms in five pn alleles are localized within a 1.2-kilobase genomic fragment, of which only transcription unit II is a part. The cDNA of this unit recognizes 1.65- and 1.8-kilobase messages in wild-type Drosophila adult head and body tissues that are absent or extremely reduced in pn mutants. Taken together, the results suggest that transcription unit II defines a part of the pn locus and its cDNA encodes a putative structural gene of pn.

摘要

果蝇黑腹果蝇的梅干(pn)基因座与梅干杀手基因座之间的互补致死相互作用是一种不寻常且高度特异的现象。pn基因的损伤会导致复眼呈现棕紫色,而条件显性的梅干杀手基因突变本身没有表型。然而,携带一份梅干杀手基因的半合子或纯合子pn突变体在幼虫发育的第二至第三龄后期死亡。作为理解这种致死性的分子本质以及pn在色素生物合成中作用的一步,我们利用P元件诱导的等位基因pn38中的转座子标签克隆了pn基因座。此外,通过转座子在pn38中的重新移动产生了七个独立的回复系。pn基因位于一个转录活跃的区域,与该区域对应的分离cDNA分为三个转录单元:I、II和III。Southern分析表明,五个pn等位基因中的限制性片段长度多态性位于一个1.2千碱基的基因组片段内,其中只有转录单元II是其一部分。该单元的cDNA在野生型果蝇成虫头部和身体组织中识别出1.65和1.8千碱基的信使RNA,而在pn突变体中则不存在或极度减少。综合来看,这些结果表明转录单元II定义了pn基因座的一部分,其cDNA编码了一个假定的pn结构基因。

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