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构建用于单个野生甜菜着丝粒分子剖析和甜菜(Beta vulgaris)基因组分析的BAC文库并进行表征。

Construction and characterization of a BAC library for the molecular dissection of a single wild beet centromere and sugar beet (Beta vulgaris) genome analysis.

作者信息

Gindullis F, Dechyeva D, Schmidt T

机构信息

CelITec GmbH Biotechnologie, Hamburg, Germany.

出版信息

Genome. 2001 Oct;44(5):846-55.

Abstract

We have constructed a sugar beet bacterial artificial chromosome (BAC) library of the chromosome mutant PRO1. This Beta vulgaris mutant carries a single chromosome fragment of 6-9 Mbp that is derived from the wild beet Beta procumbens and is transmitted efficiently in meiosis and mitosis. The library consists of 50,304 clones, with an average insert size of 125 kb. Filter hybridizations revealed that approximately 3.1% of the clones contain mitochondrial or chloroplast DNA. Based on a haploid genome size of 758 Mbp, the library represents eight genome equivalents. Thus, there is a greater than 99.96% probability that any sequence of the PROI genome can be found in the library. Approximately 0.2% of the clones hybridized with centromeric sequences of the PRO1 minichromosome. Using the identified BAC clones in fluorescence in situ hybridization experiments with PRO1 and B. procumbens chromosome spreads, their wild-beet origin and centromeric localization were demonstrated. Comparative Southern hybridization of pulsed-field separated PROI DNA and BAC inserts indicate that the centromeric region of the minichromosome is represented by overlapping clones in the library. Therefore, the PRO1 BAC library provides a useful tool for the characterization of a single plant centromere and is a valuable resource for sugar beet genome analysis.

摘要

我们构建了染色体突变体PRO1的甜菜细菌人工染色体(BAC)文库。这种甜菜突变体携带一个6 - 9兆碱基对的单一染色体片段,该片段源自野生甜菜平卧甜菜,并且在减数分裂和有丝分裂中能高效传递。该文库由50304个克隆组成,平均插入片段大小为125千碱基对。滤膜杂交显示,约3.1%的克隆含有线粒体或叶绿体DNA。基于单倍体基因组大小758兆碱基对,该文库代表八个基因组当量。因此,在文库中找到PROI基因组任何序列的概率大于99.96%。约0.2%的克隆与PRO1小染色体的着丝粒序列杂交。在与PRO1和平卧甜菜染色体铺片的荧光原位杂交实验中使用已鉴定的BAC克隆,证实了它们的野生甜菜起源和着丝粒定位。脉冲场分离的PROI DNA和BAC插入片段的比较Southern杂交表明,小染色体的着丝粒区域由文库中重叠的克隆代表。因此,PRO1 BAC文库为单个植物着丝粒的表征提供了有用工具,并且是甜菜基因组分析的宝贵资源。

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