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果蝇中缺口分割基因驼背基因的鉴定与表达

Identification and expression of the gap segmentation gene hunchback in Drosophila melanogaster.

作者信息

Bender M, Horikami S, Cribbs D, Kaufman T C

机构信息

Department of Biology, Indiana University, Bloomington 47401.

出版信息

Dev Genet. 1988;9(6):715-32. doi: 10.1002/dvg.1020090604.

DOI:10.1002/dvg.1020090604
PMID:2849517
Abstract

Genetic analysis has shown that the gap segmentation gene hunchback (hb) is a member of the genetic hierarchy involved in pattern formation in Drosophila. To identify the hb gene, we have mapped the position of hb mutant breakpoints within a chromosomal walk of the 85A region by genomic Southern blots and determined the transcription pattern of DNA from the walk. We detect a single gene within the domain defined by breakpoint mapping. We conclude that we have identified the hunchback gene because three mutations that inactivate hb physically interrupt or delete this gene. Northern analysis shows that the hb gene gives rise to at least five overlapping transcripts ranging in length from 2.6 to 3.5 kilobases. S1 nuclease and primer extension experiments demonstrate that the gene employs two promoters and three polyadenylation sites. The two hb promoters have different temporal specificities. Transcripts arising from the upstream promoter are detected from 0-12 hours of embryogenesis as well as in adult female and male RNA preparations. Transcripts arising from the downstream promoter accumulate only from 0-6 hours of embryogenesis. During the syncytial blastoderm stage, transcripts from the hb gene accumulate over a broad anterior and a narrow posterior domain. This pattern sharpens during the late blastoderm/early gastrula stage to produce an embryo with two stripes of hybridization anterior and one stripe posterior. Later, hb transcripts are detected within the ventral hypoderm in extended germ band stage embryos.

摘要

遗传分析表明,间隙分割基因驼背(hb)是参与果蝇模式形成的遗传层次结构的成员。为了鉴定hb基因,我们通过基因组Southern印迹法在85A区域的染色体步移中定位了hb突变断点的位置,并确定了该步移中DNA的转录模式。我们在断点定位所定义的区域内检测到一个单一基因。我们得出结论,我们已经鉴定出驼背基因,因为三个使hb失活的突变在物理上中断或删除了该基因。Northern分析表明,hb基因产生至少五种重叠转录本,长度范围为2.6至3.5千碱基。S1核酸酶和引物延伸实验表明,该基因使用两个启动子和三个聚腺苷酸化位点。两个hb启动子具有不同的时间特异性。来自上游启动子的转录本在胚胎发育的0至12小时以及成年雌性和雄性RNA制剂中被检测到。来自下游启动子的转录本仅在胚胎发育的0至6小时积累。在合胞体胚盘阶段,hb基因的转录本在前部广泛区域和后部狭窄区域积累。这种模式在胚盘后期/原肠胚早期阶段变得更加明显,产生一个具有两条前部杂交带和一条后部杂交带的胚胎。后来,在延伸胚带阶段的胚胎中,在腹侧皮下组织中检测到hb转录本。

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