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菜豆的分子细胞遗传学:18S-5.8S-25S rRNA 基因、5S rRNA 基因、端粒样序列和一组着丝粒重复 DNA 序列的物理组织和特征。

The molecular cytogenetics of Vigna unguiculata (L.) Walp: the physical organization and characterization of 18s-5.8s-25s rRNA genes, 5s rRNA genes, telomere-like sequences, and a family of centromeric repetitive DNA sequences.

机构信息

Istituto del Germoplasma, CNR, Via G. Amendola 165/A, 70126, Bari, Italy.

出版信息

Theor Appl Genet. 1995 Nov;91(6-7):928-35. doi: 10.1007/BF00223902.

DOI:10.1007/BF00223902
PMID:24169979
Abstract

A knowledge of genome organization is important for understanding how genomes function and evolve, and provide information likely to be useful in plant breeding programmes involving hybridization and genetic manipulation. Molecular techniques, including in situ hybridization, molecular cloning and DNA sequencing, are proving valuable tools to investigate the structure, organization, and diversity of chromosomes in agricultural crops. Heterologous labelled 18 s-5.8 s-25 s (pTa71) and 5 s rDNAs (pTa794) were used for in situ hybridization on Vigna unguiculata (L.) Walp. chromosomes. Hybridization with 18 s-5.8 s-25 s rRNA gene probes occurred at the same chromosomal sites which were positive to the CMA fluorochrome. Silver staining of nucleolar-organizing regions indicated that all the rDNA sites detected using the 18 s-5.8 s-25 s rRNA gene probe possessed active genes. Degenerate telomeric repeats gave hybridization signals at the telomeres of most chromosomes and no intercalary sites were detected at metaphase; the sequences appear to have no preferential distribution in interphase nuclei. A repetitive DraI family from V. unguiculata was cloned (pVuKB1) and characterized. The DraI repeat is 488 nucleotides long, AT rich (74%), and hybridized on all chromosomes in the centromeric areas. The presence of this sequence family was investigated by Southern hybridization in different Vigna species and other Leguminoseae. It was only detected in V. unguiculata, and hence represents a species-specific DNA sequence.

摘要

基因组结构的知识对于理解基因组的功能和进化非常重要,并为涉及杂交和遗传操作的植物育种计划提供了可能有用的信息。包括原位杂交、分子克隆和 DNA 测序在内的分子技术被证明是研究农业作物染色体结构、组织和多样性的有用工具。异源标记的 18s-5.8s-25s(pTa71)和 5s rDNA(pTa794)被用于豇豆(Vigna unguiculata(L.)Walp.)染色体的原位杂交。18s-5.8s-25s rRNA 基因探针的杂交发生在与 CMA 荧光染料呈阳性的相同染色体位点。核仁组织区域的银染表明,使用 18s-5.8s-25s rRNA 基因探针检测到的所有 rDNA 位点都具有活性基因。退化的端粒重复序列在大多数染色体的端粒处产生杂交信号,在中期没有检测到居间位点;这些序列似乎在间期核中没有优先分布。从豇豆克隆并表征了一个重复的 DraI 家族(pVuKB1)。DraI 重复序列长 488 个核苷酸,富含 AT(74%),并在着丝粒区的所有染色体上杂交。Southern 杂交研究了不同的豇豆种和其他豆科植物中该序列家族的存在情况。它仅在豇豆中被检测到,因此代表了一种物种特异性的 DNA 序列。

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