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矮牵牛二元细菌人工染色体文库的构建以及与自交不亲和(S-)位点连锁的大基因组片段的分离。

Construction of a binary bacterial artificial chromosome library of Petunia inflata and the isolation of large genomic fragments linked to the self-incompatibility (S-) locus.

作者信息

McCubbin A G, Zuniga C, Kao T

机构信息

Department of Biochemistry and Molecular Biology, The Pennsylvania State University, University Park 16802, USA.

出版信息

Genome. 2000 Oct;43(5):820-6.

PMID:11081972
Abstract

The Solanaceae family of flowering plants possesses a type of self-incompatibility mechanism that enables the pistil to reject self pollen but accept non-self pollen for fertilization. The pistil function in this system has been shown to be controlled by a polymorphic gene at the S-locus, termed the S-RNase gene. The pollen function is believed to be controlled by another as yet unidentified polymorphic gene at the S-locus, termed the pollen S-gene. As a first step in using a functional genomic approach to identify the pollen S-gene, a genomic BAC (bacterial artificial chromosome) library of the S2S2 genotype of Petunia inflata, a self-incompatible solanaceous species, was constructed using a Ti-plasmid based BAC vector, BIBAC2. The average insert size was 136.4 kb and the entire library represented a 7.5-fold genome coverage. Screening of the library using cDNAs for the S2-RNase gene and 13 pollen-expressed genes that are linked to the S-locus yielded 51 positive clones, with at least one positive clone for each gene. Collectively, at least 2 Mb of the chromosomal region was spanned by these clones. Together, three clones that contained the S2-RNase gene spanned approximately 263 kb. How this BAC library and the clones identified could be used to identify the pollen S-gene and to study other aspects of self-incompatibility is discussed.

摘要

开花植物茄科拥有一种自交不亲和机制,该机制能使雌蕊排斥自身花粉,但接受非自身花粉进行受精。在这个系统中,雌蕊的功能已被证明受S位点上一个多态性基因控制,该基因被称为S-RNase基因。花粉的功能据信受S位点上另一个尚未确定的多态性基因控制,该基因被称为花粉S基因。作为使用功能基因组学方法鉴定花粉S基因的第一步,利用基于Ti质粒的BAC载体BIBAC2构建了自交不亲和茄科植物矮牵牛S2S2基因型的基因组BAC(细菌人工染色体)文库。平均插入片段大小为136.4 kb,整个文库代表7.5倍的基因组覆盖率。用S2-RNase基因的cDNA和13个与S位点连锁的花粉表达基因筛选该文库,得到51个阳性克隆,每个基因至少有一个阳性克隆。这些克隆总共覆盖了至少2 Mb的染色体区域。包含S2-RNase基因的三个克隆一起覆盖了大约263 kb。本文讨论了如何利用这个BAC文库和鉴定出的克隆来鉴定花粉S基因以及研究自交不亲和的其他方面。

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