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小鼠马珠蛋白-4基因的特征:与编码转录因子RBP-1的基因存在5'端反向重叠。

Characterization of the mouse matrilin-4 gene: a 5' antiparallel overlap with the gene encoding the transcription factor RBP-l.

作者信息

Wagener R, Kobbe B, Aszódi A, Aeschlimann D, Paulsson M

机构信息

Institute for Biochemistry, Medical Faculty, University of Cologne, Joseph-Stelzmann-Str. 52, Cologne, D-50931, Germany.

出版信息

Genomics. 2001 Aug;76(1-3):89-98. doi: 10.1006/geno.2001.6589.

DOI:10.1006/geno.2001.6589
PMID:11549321
Abstract

We have isolated and characterized the gene encoding mouse matrilin-4 (Matn4), an extracellular matrix protein present in a broad spectrum of tissues. The gene spanned 16 kb, consisted of 12 exons, and localized to chromosome 2. As in all known matrilin genes, the last intron, separating the exons coding for the coiled-coil domain, did not follow the GT-AG rule and belonged to the subgroup of introns having AT-AC at the ends. Matn4 contained two exons in the 5' UTR that could be alternatively spliced. We localized a major and a minor transcription start site to two different untranslated exons: exon 0a and exon 0b. Matn4 divergently overlapped 5' with the gene encoding RBP-L (for recombining binding protein suppressor of hairless-like; Rbpsuhl), a transcription factor with homology to RBP-JK. Exon 1 of Rbpsuhl was located in the second intron of Matn4, whereas exon 0a, the first exon of Matn4, was located in the second intron of Rbpsuhl. The second exons of the respective genes overlapped in an antisense orientation. We mapped the major transcription start of Rbpsuhl to a position approximately 150 nt upstream of the splice acceptor site of the first intron, leading to the synthesis of a truncated variant of RBP-L probably missing the amino-terminal 121 amino acid residues. We analyzed the expression of the different Matn4 and Rbpsuhl transcripts by quantitative RT-PCR; this showed the highest expression for both genes in lung and brain. In situ hybridization of brain sections showed a partially overlapping expression pattern for the two genes.

摘要

我们已经分离并鉴定了编码小鼠马替林-4(Matn4)的基因,Matn4是一种存在于多种组织中的细胞外基质蛋白。该基因跨度为16 kb,由12个外显子组成,定位于2号染色体。与所有已知的马替林基因一样,分隔编码卷曲螺旋结构域的外显子的最后一个内含子不遵循GT-AG规则,属于末端具有AT-AC的内含子亚组。Matn4在5'非翻译区(UTR)包含两个可选择性剪接的外显子。我们将一个主要和一个次要转录起始位点定位到两个不同的非翻译外显子:外显子0a和外显子0b。Matn4在5'端与编码RBP-L(重组结合蛋白无毛样抑制因子;Rbpsuhl)的基因发散性重叠,RBP-L是一种与RBP-JK具有同源性的转录因子。Rbpsuhl的外显子1位于Matn4的第二个内含子中,而Matn4的第一个外显子外显子0a位于Rbpsuhl的第二个内含子中。各自基因的第二个外显子以反义方向重叠。我们将Rbpsuhl的主要转录起始位点定位到第一个内含子剪接受体位点上游约150 nt处,导致合成可能缺失氨基末端121个氨基酸残基的RBP-L截短变体。我们通过定量逆转录-聚合酶链反应(RT-PCR)分析了不同Matn4和Rbpsuhl转录本的表达;结果显示这两个基因在肺和脑中表达最高。脑切片的原位杂交显示这两个基因的表达模式部分重叠。

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