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Molecular Cloning and Duplication of the Nematode Sex-Determining Gene Tra-1

机译:线虫性别决定基因Tra-1的分子克隆和复制。

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摘要

The autosomal sex-determining gene tra-1 plays a major role in controlling sexual phenotype in the nematode Caenorhabditis elegans. This gene is the terminal global regulator in a well-characterized cascade of sex-determining genes. It governs all aspects of somatic sexual differentiation, and it also has important functions in governing germ-line differentiation. Previous genetic analyses have led to the characterization of many loss-of-function (masculinizing) and gain-of-function (dominant feminizing) alleles, and to models for the functions and regulation of tra-1. The gene was cloned by identifying linked transposon insertions, about 200 kb away from tra-1. From this starting point a series of YAC, cosmid and phage clones were assembled into a genomic walk covering over 400 kb. Much of this region was found to be unrepresented in the cosmid database that covers most of the C. elegans genome. This deficit is largely or wholly due to the presence of sequences that cannot be cloned in rec(+)bacterial hosts. The ratio of physical map distances to recombinational map distances in the tra-1 region of the genome appears to be unusually low, indicating considerable local map expansion. The location of tra-1 within the cloned region was determined using a variety of tra-1 mutations that are associated with physical rearrangements of the gene. One of these is a 14-kb deletion, which behaves as a null allele. Another rearrangement, eDp24, is a tandem duplication of 22 kb. Genetic analysis demonstrates that eDp24 carries two incomplete copies of tra-1, and that these copies appear to interact, suggesting some form of negative autoregulation at this locus. Three variant forms of the tra-1 locus have been identified in different natural isolates of C. elegans.
机译:常染色体性别决定基因tra-1在线虫秀丽隐杆线虫的控制性表型中起主要作用。该基因是性别决定性基因的一个很好表征的级联中的末端全局调节子。它控制体细胞性别分化的各个方面,并且在控制种系分化中也具有重要的功能。以前的遗传分析导致许多功能丧失(男性化)和功能获得(女性占主导)等位基因的表征,以及tra-1的功能和调控模型。通过鉴定距离tra-1约200 kb的连锁转座子插入来克隆该基因。从这个起点开始,将一系列YAC,粘粒和噬菌体克隆组装成一个覆盖400 kb以上的基因组序列。发现覆盖大部分秀丽隐杆线虫基因组的粘粒数据库中未显示该区域的大部分。这种缺陷主要或完全是由于无法克隆到rec(+)细菌宿主中的序列的存在。基因组tra-1区域中物理图谱距离与重组图谱距离的比值似乎异常低,表明局部图谱扩展相当大。使用与基因的物理重排相关的多种tra-1突变来确定tra-1在克隆区域内的位置。其中之一是14kb缺失,表现为无效等位基因。另一个重排,eDp24,是22 kb的串联重复。遗传分析表明eDp24携带两个不完整的tra-1拷贝,并且这些拷贝似乎相互作用,表明在该基因座存在某种形式的负自动调节。在秀丽隐杆线虫的不同天然分离物中已鉴定出tra-1基因座的三种变体形式。

著录项

  • 期刊名称 Genetics
  • 作者

    J. Hodgkin;

  • 作者单位
  • 年(卷),期 1993(133),3
  • 年度 1993
  • 页码 543–560
  • 总页数 18
  • 原文格式 PDF
  • 正文语种
  • 中图分类 遗传学;
  • 关键词

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