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小鼠犁鼻器受体基因的序列多样性与基因组组织

Sequence diversity and genomic organization of vomeronasal receptor genes in the mouse.

作者信息

Del Punta K, Rothman A, Rodriguez I, Mombaerts P

机构信息

The Rockefeller University, New York, New York 10021, USA.

出版信息

Genome Res. 2000 Dec;10(12):1958-67. doi: 10.1101/gr.10.12.1958.

Abstract

The vomeronasal system of mice is thought to be specialized in the detection of pheromones. Two multigene families have been identified that encode proteins with seven putative transmembrane domains and that are expressed selectively in subsets of neurons of the vomeronasal organ. The products of these vomeronasal receptor (Vr) genes are regarded as candidate pheromone receptors. Little is known about their genomic organization and sequence diversity, and only five sequences of mouse V1r coding regions are publicly available. Here, we have begun to characterize systematically the V1r repertoire in the mouse. We isolated 107 bacterial artificial chromosomes (BACs) containing V1r genes from a 129 mouse library. Hybridization experiments indicate that at least 107 V1r-like sequences reside on these BACs. We assembled most of the BACs into six contigs, of which one major contig and one minor contig were characterized in detail. The major contig is 630-860 kb long, encompasses a cluster of 21-48 V1r genes, and contains marker D6Mit227. Sequencing of the coding regions was facilitated by the absence of introns. We determined the sequence of the coding region of 25 possibly functional V1r genes and seven pseudogenes. The functional V1rs can be arranged into three groups; V1rs of one group are novel and substantially divergent from the other V1rs. The genomic and sequence information described here should be useful in defining the biological function of these receptors.

摘要

小鼠的犁鼻系统被认为专门用于检测信息素。已鉴定出两个多基因家族,它们编码具有七个推定跨膜结构域的蛋白质,并在犁鼻器神经元亚群中选择性表达。这些犁鼻受体(Vr)基因的产物被视为候选信息素受体。关于它们的基因组组织和序列多样性知之甚少,目前仅有五条小鼠V1r编码区序列公开可用。在此,我们开始系统地表征小鼠中的V1r基因库。我们从一个129小鼠文库中分离出107个含有V1r基因的细菌人工染色体(BAC)。杂交实验表明,这些BAC上至少存在107个V1r样序列。我们将大部分BAC组装成六个重叠群,其中一个主要重叠群和一个次要重叠群得到了详细表征。主要重叠群长度为630 - 860 kb,包含一个由21 - 48个V1r基因组成的簇,并含有标记D6Mit227。编码区由于没有内含子而便于测序。我们确定了25个可能具有功能的V1r基因和7个假基因的编码区序列。功能性V1r可分为三组;其中一组V1r是新的,与其他V1r有很大差异。这里描述的基因组和序列信息应有助于确定这些受体的生物学功能。

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本文引用的文献

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