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MIWI and piRNA-mediated cleavage of messenger RNAs in mouse testes

The piRNA machinery is known for its role in mediating epigenetic silencing of transposons. Recent studies suggest that this function also involves piRNA-guided cleavage of transposon-derived transcripts. As many piRNAs also appear to have the capacity to target diverse mRNAs, this raises the intrig...

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Autores principales: Zhang, Peng, Kang, Jun-Yan, Gou, Lan-Tao, Wang, Jiajia, Xue, Yuanchao, Skogerboe, Geir, Dai, Peng, Huang, Da-Wei, Chen, Runsheng, Fu, Xiang-Dong, Liu, Mo-Fang, He, Shunmin
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Nature Publishing Group 2015
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4650574/
https://www.ncbi.nlm.nih.gov/pubmed/25582079
http://dx.doi.org/10.1038/cr.2015.4
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author Zhang, Peng
Kang, Jun-Yan
Gou, Lan-Tao
Wang, Jiajia
Xue, Yuanchao
Skogerboe, Geir
Dai, Peng
Huang, Da-Wei
Chen, Runsheng
Fu, Xiang-Dong
Liu, Mo-Fang
He, Shunmin
author_facet Zhang, Peng
Kang, Jun-Yan
Gou, Lan-Tao
Wang, Jiajia
Xue, Yuanchao
Skogerboe, Geir
Dai, Peng
Huang, Da-Wei
Chen, Runsheng
Fu, Xiang-Dong
Liu, Mo-Fang
He, Shunmin
author_sort Zhang, Peng
collection PubMed
description The piRNA machinery is known for its role in mediating epigenetic silencing of transposons. Recent studies suggest that this function also involves piRNA-guided cleavage of transposon-derived transcripts. As many piRNAs also appear to have the capacity to target diverse mRNAs, this raises the intriguing possibility that piRNAs may act extensively as siRNAs to degrade specific mRNAs. To directly test this hypothesis, we compared mouse PIWI (MIWI)-associated piRNAs with experimentally identified cleaved mRNA fragments from mouse testes, and observed cleavage sites that predominantly occur at position 10 from the 5′ end of putative targeting piRNAs. We also noted strong biases for U and A residues at nucleotide positions 1 and 10, respectively, in both piRNAs and mRNA fragments, features that resemble the pattern of piRNA amplification by the 'ping-pong' cycle. Through mapping of MIWI-RNA interactions by CLIP-seq and gene expression profiling, we found that many potential piRNA-targeted mRNAs directly interact with MIWI and show elevated expression levels in the testes of Miwi catalytic mutant mice. Reporter-based assays further revealed the importance of base pairing between piRNAs and mRNA targets and the requirement for both the slicer activity and piRNA-loading ability of MIWI in piRNA-mediated target repression. Importantly, we demonstrated that proper turnover of certain key piRNA targets is essential for sperm formation. Together, these findings reveal the siRNA-like function of the piRNA machinery in mouse testes and its central requirement for male germ cell development and maturation.
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spelling pubmed-46505742015-12-01 MIWI and piRNA-mediated cleavage of messenger RNAs in mouse testes Zhang, Peng Kang, Jun-Yan Gou, Lan-Tao Wang, Jiajia Xue, Yuanchao Skogerboe, Geir Dai, Peng Huang, Da-Wei Chen, Runsheng Fu, Xiang-Dong Liu, Mo-Fang He, Shunmin Cell Res Original Article The piRNA machinery is known for its role in mediating epigenetic silencing of transposons. Recent studies suggest that this function also involves piRNA-guided cleavage of transposon-derived transcripts. As many piRNAs also appear to have the capacity to target diverse mRNAs, this raises the intriguing possibility that piRNAs may act extensively as siRNAs to degrade specific mRNAs. To directly test this hypothesis, we compared mouse PIWI (MIWI)-associated piRNAs with experimentally identified cleaved mRNA fragments from mouse testes, and observed cleavage sites that predominantly occur at position 10 from the 5′ end of putative targeting piRNAs. We also noted strong biases for U and A residues at nucleotide positions 1 and 10, respectively, in both piRNAs and mRNA fragments, features that resemble the pattern of piRNA amplification by the 'ping-pong' cycle. Through mapping of MIWI-RNA interactions by CLIP-seq and gene expression profiling, we found that many potential piRNA-targeted mRNAs directly interact with MIWI and show elevated expression levels in the testes of Miwi catalytic mutant mice. Reporter-based assays further revealed the importance of base pairing between piRNAs and mRNA targets and the requirement for both the slicer activity and piRNA-loading ability of MIWI in piRNA-mediated target repression. Importantly, we demonstrated that proper turnover of certain key piRNA targets is essential for sperm formation. Together, these findings reveal the siRNA-like function of the piRNA machinery in mouse testes and its central requirement for male germ cell development and maturation. Nature Publishing Group 2015-02 2015-01-13 /pmc/articles/PMC4650574/ /pubmed/25582079 http://dx.doi.org/10.1038/cr.2015.4 Text en Copyright © 2015 Shanghai Institutes for Biological Sciences, Chinese Academy of Sciences http://creativecommons.org/licenses/by-nc-nd/3.0 This work is licensed under the Creative Commons Attribution-NonCommercial-No Derivative Works 3.0 Unported License. To view a copy of this license, visit http://creativecommons.org/licenses/by-nc-nd/3.0
spellingShingle Original Article
Zhang, Peng
Kang, Jun-Yan
Gou, Lan-Tao
Wang, Jiajia
Xue, Yuanchao
Skogerboe, Geir
Dai, Peng
Huang, Da-Wei
Chen, Runsheng
Fu, Xiang-Dong
Liu, Mo-Fang
He, Shunmin
MIWI and piRNA-mediated cleavage of messenger RNAs in mouse testes
title MIWI and piRNA-mediated cleavage of messenger RNAs in mouse testes
title_full MIWI and piRNA-mediated cleavage of messenger RNAs in mouse testes
title_fullStr MIWI and piRNA-mediated cleavage of messenger RNAs in mouse testes
title_full_unstemmed MIWI and piRNA-mediated cleavage of messenger RNAs in mouse testes
title_short MIWI and piRNA-mediated cleavage of messenger RNAs in mouse testes
title_sort miwi and pirna-mediated cleavage of messenger rnas in mouse testes
topic Original Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4650574/
https://www.ncbi.nlm.nih.gov/pubmed/25582079
http://dx.doi.org/10.1038/cr.2015.4
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