文化大學機構典藏 CCUR:Item 987654321/20527
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    Please use this identifier to cite or link to this item: https://irlib.pccu.edu.tw/handle/987654321/20527


    Title: Transcription of the rat testis-specific Rtdpoz-T1 and-T2 retrogenes during embryo development: co-transcription and frequent exonisation of transposable element sequences
    Authors: Huang, CJ (Huang, Chiu-Jung)
    Lin, WY (Lin, Wan-Yi)
    Chang, CM (Chang, Che-Ming)
    Choo, KB (Choo, Kong-Bung)
    Contributors: 動物科學系
    Date: 2009
    Issue Date: 2011-11-30 14:01:30 (UTC+8)
    Abstract: Background: Retrotransposition is an important evolutionary force for the creation of new and potentially functional intronless genes which are collectively called retrogenes. Many retrogenes are expressed in the testis and the gene products have been shown to actively participate in spermatogenesis and other unique functions of the male germline. We have previously reported a cluster of retrogenes in the rat genome that encode putative TRAF- and POZ-domain proteins. Two of the genes, Rtdpoz-T1 and -T2 (abbreviated as T1 and T2), have further been shown to be expressed specifically in the rat testis.

    Results: We show here that the T1 and T2 genes are also expressed in the rat embryo up to days 16-17 of development when the genes are silenced until being re-activated in the adult testis. On database interrogation, we find that some T1/T2 exons are chromosomally duplicated as cassettes of 2 or 3 exons consistent with retro-duplication. The embryonic T1/T2 transcripts, characterised by RT-PCR-cloning and rapid amplification of cDNA ends, are further found to have acquired one or more noncoding exons in the 5'-untranslated region (5'-UTR). Most importantly, the T1/T2 locus is embedded within a dense field of relics of transposable element (TE) derived mainly from LINE1 and ERV sequences, and the TE sequences are frequently exonised through alternative splicing to form the 5'-UTR sequences of the T1/T2 transcripts. In a case of T1 transcript, the 3'-end is extended into and terminated within an L1 sequence. Since the two genes share a common exon 1 and are, therefore, regulated by a single promoter, a T2-to-T1 co-transcription model is proposed. We further demonstrate that the exonised 5'-UTR TE sequences could lead to the creation of upstream open reading frames resulting in translational repression.

    Conclusion: Exonisation of TE sequences is a frequent event in the transcription of retrogenes during embryonic development and in the testis and may contribute to post-transcriptional regulation of expression of retrogenes.
    Appears in Collections:[Department of Animal Science] journal articles

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