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秀丽隐杆线虫中ama-1的精细结构遗传学,ama-1是一个编码RNA聚合酶II的鹅膏蕈碱结合亚基的必需基因。

Fine-structure genetics of ama-1, an essential gene encoding the amanitin-binding subunit of RNA polymerase II in Caenorhabditis elegans.

作者信息

Bullerjahn A M, Riddle D L

机构信息

Division of Biological Sciences, University of Missouri, Columbia 65211.

出版信息

Genetics. 1988 Oct;120(2):423-34. doi: 10.1093/genetics/120.2.423.

Abstract

A fine-structure genetic map has been constructed for ama-1 IV, an essential gene in Caenorhabditis elegans encoding the amanitin-binding subunit of RNA polymerase II. Sixteen EMS-induced recessive-lethal mutations have been positioned in the gene by determining their intragenic recombination frequencies with m118, a mutation that confers dominant resistance to alpha-amanitin. The 16 mutants, all isolated in the ama-1(m118) background, include 13 that are early larval lethals, and three that are mid-larval lethals, at 25 degrees. Six of the mutants exhibit temperature-dependence in the severity of their phenotype. Intragenic recombination between the lethal site and the parental resistance mutation was detected by means of resistance to amanitin. Recombinants were detected at frequencies as low as 2 X 10(-6). The segregation of the closely linked flanking markers, unc-17 and unc-5, revealed whether the lethal mutation was to the left or the right of m118. By adding the distances between the extreme left and right mutations, the ama-1 gene is estimated to be 0.011 map unit long, with m118 positioned 0.004 map unit from the left-most lethal mutation. To order the lethal mutations with respect to each other, viable heteroallelic strains were constructed using the free duplication, mDp1[unc-17(e113) dpy-13(+) ama-1(+)]. The heteroallelic strains were sensitive to amanitin, and recombination events between the lethal mutations were specifically selected by means of the dominant amanitin resistance encoded on the recombinant chromosome. The segregation of outside markers revealed the left-right order of the lethal mutations. The position of mutations within the gene is nonrandom. Functional domains of the ama-1 gene indicated by the various lethal phenotypes are discussed.

摘要

已构建秀丽隐杆线虫中一个必需基因ama-1 IV的精细结构遗传图谱,该基因编码RNA聚合酶II的鹅膏蕈碱结合亚基。通过测定16个经EMS诱导的隐性致死突变与m118(一种赋予对α-鹅膏蕈碱显性抗性的突变)的基因内重组频率,将这些突变定位在该基因中。所有16个突变体均在ama-1(m118)背景下分离得到,其中13个是早期幼虫致死突变体,3个是中期幼虫致死突变体,温度为25摄氏度。6个突变体的表型严重程度表现出温度依赖性。通过对鹅膏蕈碱的抗性检测致死位点与亲本抗性突变之间的基因内重组。重组体的检测频率低至2×10(-6)。紧密连锁的侧翼标记unc-17和unc-5的分离揭示了致死突变位于m118的左侧还是右侧。通过累加最左侧和最右侧突变之间的距离,估计ama-1基因长度为0.011个图距单位,m118距最左侧致死突变0.004个图距单位。为了确定致死突变之间的相对顺序,利用自由重复mDp1[unc-17(e113) dpy-13(+) ama-1(+)]构建了有活力的异等位基因菌株。这些异等位基因菌株对鹅膏蕈碱敏感,通过重组染色体上编码的显性鹅膏蕈碱抗性特异性选择致死突变之间的重组事件。外部标记的分离揭示了致死突变的左右顺序。讨论了由各种致死表型所指示的ama-1基因内突变的位置。

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