A long non-coding RNA transcribed from conserved non-coding sequences contributes to the mouse prolyl oligopeptidase gene activation

Matsubara, Shin; Kurihara, Misuzu; Kimura, Atsushi

doi:10.1093/jb/mvt113

Cited by 13 publications

(19 citation statements)

References 71 publications

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“…RACE analyses were performed as previously described (Kurihara et al, ; Matsubara et al, ). For 5′RACE, reverse transcription was performed with RT‐1 primer, and the first PCR was performed with GSP1 and the Abridged Anchor Primer.…”

Section: Methodsmentioning

confidence: 99%

A genomic region transcribed into a long noncoding RNA interacts with the Prss42/Tessp‐2 promoter in spermatocytes during mouse spermatogenesis, and its flanking sequences can function as enhancers

Yoneda

Satoh

Yoshida

et al. 2016

Molecular Reproduction Devel

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SUMMARYSpermatogenesis is precisely regulated by many meiotic stage-specific genes, but their regulatory mechanisms are not fully understood. The Prss/Tessp gene cluster is located on the mouse chromosome 9F2-F3, and the three genes, Prss42/Tessp-2, Prss43/Tessp-3, and Prss44/Tessp-4 on the cluster, are specifically activated in pachytene spermatocytes during meiosis. To elucidate a mechanism of their activation, we searched for DNase I hypersensitive sites (HSs) and long noncoding RNAs (lncRNAs) at the Prss/Tessp locus. We found eight DNase I HSs, three of which were testicular germ cell-specific at or close to the Prss42/Tessp-2 promoter, and a testis-specific lncRNA, lncRNA-HSVIII, which was transcribed from 3' to the Prss42/Tessp-2 gene. By in situ hybridization, lncRNA-HSVIII was localized in nuclei of most pachytene spermatocytes and in cytosols of pachytene spermatocytes at stage X and spermatids. Chromosome conformation capture assay showed that the chromatin at lncRNA-HSVIII specifically interacted with the Prss42/Tessp-2 promoter in primary and secondary spermatocytes. By reporter gene assay, a 5.8-kb genome sequence, encompassing the entire lncRNA-HSVIII sequence and its flanking regions, significantly increased Prss42/Tessp-2 promoter activity, but transfection of this construct did not change the lncRNA-HSVIII expression, which indicated that the increased promoter activity was likely to be dependent on enhancer activity. Indeed, we found that both upstream and downstream regions of the lncRNA-HSVIII sequence significantly increased Prss42/Tessp-2 promoter activity. Our data indicate the direct interaction of a genomic region at lncRNA-HSVIII with the Prss42/Tessp-2 promoter in spermatocytes and suggest that adjacent sequences to the lncRNA function as enhancers for the Prss42/Tessp-2 gene.4

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Section: Methodsmentioning

confidence: 99%

A genomic region transcribed into a long noncoding RNA interacts with the Prss42/Tessp‐2 promoter in spermatocytes during mouse spermatogenesis, and its flanking sequences can function as enhancers

Yoneda

Satoh

Yoshida

et al. 2016

Molecular Reproduction Devel

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“…Total RNAs from the human liver and testis were purchased from Clontech Laboratories, Inc. (Mountain View, USA) and reverse transcription‐polymerase chain reaction (RT‐PCR) was done as previously described [17]. Primer sequences are shown in Table 1 .…”

Section: Methodsmentioning

confidence: 99%

“…5′RACE and 3′RACE were performed as previously described [7,17]. All the amplified products were subcloned into a pBluescript vector (Stratagene, La Jolla, CA) by the TA‐cloning method, and at least 10 subclones were sequenced for each product.…”

Section: Methodsmentioning

confidence: 99%

Characterization of the human TCAM1P pseudogene and its activation by a potential dual promoter–enhancer: Comparison with a protein‐coding mouse orthologue

Kurihara

Kimura

2015

FEBS Letters

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a b s t r a c tTCAM1P is a unitary pseudogene, which was disabled since the human-mouse divergence. Here we found that TCAM1P was specifically expressed in the human testis, with different cell type-specificity from mouse Tcam1, and characterized its transcripts. At the mouse locus, a multifunctional dual promoter-enhancer (DPE) controls the expression of Tcam1 and Smarcd2 genes. The corresponding human sequence was found to potentially function as a DPE, although the molecular mechanism was different from mouse. Interestingly, the change in DPE activity occurred before pseudogenization of TCAM1P. These data suggest the presence of a DPE in the human genome for the first time, and provide an important model of evolutionary changes in the regulatory mechanism of a pseudogene.

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“…Total RNAs were prepared and qRT-PCR was performed as previously described [14,33]. All the data were normalized to Aip.…”

Section: Quantitative Reverse-transcription-polymerase Chain Reactionmentioning

confidence: 99%

Mouse prolyl oligopeptidase plays a role in trophoblast stem cell differentiation into trophoblast giant cell and spongiotrophoblast

2017

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A long non-coding RNA transcribed from conserved non-coding sequences contributes to the mouse prolyl oligopeptidase gene activation

Cited by 13 publications

References 71 publications

A genomic region transcribed into a long noncoding RNA interacts with the Prss42/Tessp‐2 promoter in spermatocytes during mouse spermatogenesis, and its flanking sequences can function as enhancers

A genomic region transcribed into a long noncoding RNA interacts with the Prss42/Tessp‐2 promoter in spermatocytes during mouse spermatogenesis, and its flanking sequences can function as enhancers

Characterization of the human TCAM1P pseudogene and its activation by a potential dual promoter–enhancer: Comparison with a protein‐coding mouse orthologue

Mouse prolyl oligopeptidase plays a role in trophoblast stem cell differentiation into trophoblast giant cell and spongiotrophoblast

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