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豌豆(Pisum sativum L.)中重复DNA的分子和细胞遗传学分析。

Molecular and cytogenetic analysis of repetitive DNA in pea (pisum sativum L.).

作者信息

Neumann P, Nouzová M, Macas J

机构信息

Institute of Plant Molecular Biology, Laboratory of Molecular Cytogenetics, Ceské Budejovice, Czech Republic.

出版信息

Genome. 2001 Aug;44(4):716-28.

PMID:11550909
Abstract

A set of pea DNA sequences representing the most abundant genomic repeats was obtained by combining several approaches. Dispersed repeats were isolated by screening a short-insert genomic library using genomic DNA as a probe. Thirty-two clones ranging from 149 to 2961 bp in size and from 1,000 to 39,000/lC in their copy number were sequenced and further characterized. Fourteen clones were identified as retrotransposon-like sequences, based on their homologies to known elements. Fluorescence in situ hybridization using clones of reverse transcriptase and integrase coding sequences as probes revealed that corresponding retroelements were scattered along all pea chromosomes. Two novel families of tandem repeats, named PisTR-A and PisTR-B, were isolated by screening a genomic DNA library with Cot-1 DNA and by employing genomic self-priming PCR, respectively. PisTR-A repeats are 211-212 bp long, their abundance is 2 x 10(4) copies/lC, and they are partially clustered in a secondary constriction of one chromosome pair with the rest of their copies dispersed on all chromosomes. PisTR-B sequences are of similar abundance (10(4) copies/lC) but differ from the "A" family in their monomer length (50 bp), high A/T content, and chromosomal localization in a limited number of discrete bands. These bands are located mainly in (sub)telomeric and pericentromeric regions. and their patterns, together with chromosome morphology, allow discrimination of all chromosome types within the pea karyotype. Whereas both tandem repeat families are mostly specific to the genus Pisum, many of the dispersed repeats were detected in other legume species, mainly those in the genus Vicia.

摘要

通过多种方法相结合,获得了一组代表豌豆基因组中最丰富重复序列的DNA序列。通过使用基因组DNA作为探针筛选短插入基因组文库来分离分散重复序列。对32个大小在149至2961 bp之间、拷贝数在1000至39000/μC之间的克隆进行了测序和进一步表征。基于与已知元件的同源性,14个克隆被鉴定为类反转录转座子序列。使用逆转录酶和整合酶编码序列的克隆作为探针进行荧光原位杂交,结果显示相应的反转录元件散布在所有豌豆染色体上。分别通过用Cot-1 DNA筛选基因组DNA文库和采用基因组自引物PCR,分离出了两个新的串联重复序列家族,命名为PisTR-A和PisTR-B。PisTR-A重复序列长度为211 - 212 bp,丰度为2×10⁴拷贝/μC,它们部分聚集在一对染色体的次缢痕处,其余拷贝分散在所有染色体上。PisTR-B序列丰度相似(10⁴拷贝/μC),但在单体长度(50 bp)、高A/T含量以及在有限数量的离散条带中的染色体定位方面与“A”家族不同。这些条带主要位于(亚)端粒和着丝粒周围区域,它们的模式与染色体形态一起,能够区分豌豆核型中的所有染色体类型。虽然这两个串联重复序列家族大多是豌豆属特有的,但在其他豆科物种中也检测到了许多分散重复序列,主要是野豌豆属中的那些。

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