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玉米粗糙叶鞘1发育突变体的遗传分析

Genetic analysis of Rough sheath1 developmental mutants of maize.

作者信息

Becraft P W, Freeling M

机构信息

Department of Plant Biology, University of California, Berkeley 94720.

出版信息

Genetics. 1994 Jan;136(1):295-311. doi: 10.1093/genetics/136.1.295.

Abstract

Maize Rough sheath1 (Rs1) mutants are dominant and cause a proliferation of sheath-like tissue at the base of the blade and throughout the ligular region. They also cause ligule displacement, a chaotic pattern of vasculature and abnormal cellular structure of vascular bundles. The affected region of Rs1-O leaves displays genetic and morphological attributes of both sheath and auricle, suggesting an overlap of these genetic programs. The rs1 locus maps approximately 26 map units distal to opaque2 (o2) on chromosome 7S, defining a new distal-most locus on the genetic map. Three mutant alleles, Rs1-O, Rs1-1025 and Rs1-Z, all display similar phenotypes. The mutations are completely dominant and the Rs1-O phenotype is not affected by dosage of the chromosome arm carrying the rs1+ allele, indicating that these alleles are neomorphic. Analysis of genetic mosaics showed that the Rs1-O phenotype is non-cell-autonomous, suggesting that intercellular signals convey the phenotype. Rs1 mutant phenotypes are affected by modifiers present in particular genetic backgrounds. An enhancer of Rs1-O was identified; segregation data imply a single recessive gene, ers1. Rs1 mutants were also found to enhance the expression of unlinked rs2 and Rs4 mutants, suggesting that these mutations affect similar developmental processes. We discuss the phenotypic and genetic similarities between Rs1 and Knotted 1 (Kn1) mutants that led to the identification of rs1 as a kn1-like homeobox gene (unpublished data).

摘要

玉米粗糙叶鞘1(Rs1)突变体为显性突变体,会导致叶片基部和整个叶舌区域的叶鞘状组织增生。它们还会导致叶舌移位、维管系统紊乱以及维管束细胞结构异常。Rs1 - O叶片的受影响区域表现出叶鞘和叶耳的遗传和形态特征,表明这些遗传程序存在重叠。rs1基因座位于7号染色体短臂上不透明2(o2)基因远端约26个遗传单位处,在遗传图谱上定义了一个新的最远端基因座。三个突变等位基因Rs1 - O、Rs1 - 1025和Rs1 - Z均表现出相似的表型。这些突变完全显性,且Rs1 - O的表型不受携带rs1 + 等位基因的染色体臂剂量的影响,表明这些等位基因是新形态的。遗传嵌合体分析表明,Rs1 - O的表型是非细胞自主的,这表明细胞间信号传递了该表型。Rs1突变体表型受特定遗传背景中存在的修饰基因影响。已鉴定出Rs1 - O的一个增强子;分离数据表明存在一个单隐性基因ers1。还发现Rs1突变体增强了不连锁的rs2和Rs4突变体的表达,这表明这些突变影响相似的发育过程。我们讨论了Rs1和结瘤1(Kn1)突变体之间的表型和遗传相似性,这些相似性导致将rs1鉴定为一个类Kn1同源异型盒基因(未发表数据)。

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