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Comparative Analysis of the miRNome of Bovine Milk Fat, Whey and Cells

Abundant miRNAs have been identified in milk and mammary gland tissues of different species. Typically, RNA in milk can be extracted from different fractions including fat, whey and cells and the mRNA transcriptome of milk could serve as an indicator of the transcriptome of mammary gland tissue. How...

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Autores principales: Li, Ran, Dudemaine, Pier-Luc, Zhao, Xin, Lei, Chuzhao, Ibeagha-Awemu, Eveline Mengwi
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2016
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4839614/
https://www.ncbi.nlm.nih.gov/pubmed/27100870
http://dx.doi.org/10.1371/journal.pone.0154129
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author Li, Ran
Dudemaine, Pier-Luc
Zhao, Xin
Lei, Chuzhao
Ibeagha-Awemu, Eveline Mengwi
author_facet Li, Ran
Dudemaine, Pier-Luc
Zhao, Xin
Lei, Chuzhao
Ibeagha-Awemu, Eveline Mengwi
author_sort Li, Ran
collection PubMed
description Abundant miRNAs have been identified in milk and mammary gland tissues of different species. Typically, RNA in milk can be extracted from different fractions including fat, whey and cells and the mRNA transcriptome of milk could serve as an indicator of the transcriptome of mammary gland tissue. However, it has not been adequately validated if the miRNA transcriptome of any milk fraction could be representative of that of mammary gland tissue. The objectives of this study were to (1) characterize the miRNA expression spectra from three milk fractions- fat, whey and cells; (2) compare miRNome profiles of milk fractions (fat, whey and cells) with mammary gland tissue miRNome, and (3) determine which milk fraction miRNome profile could be a better representative of the miRNome profile of mammary gland tissue. Milk from four healthy Canadian Holstein cows in mid lactation was collected and fractionated. Total RNA extracted from each fraction was used for library preparation followed by small RNA sequencing. In addition, miRNA transcripts of mammary gland tissues from twelve Holstein cows in our previous study were used to compare our data. We identified 210, 200 and 249 known miRNAs from milk fat, whey and cells, respectively, with 188 universally expressed in the three fractions. In addition, 33, 31 and 36 novel miRNAs from milk fat, whey and cells were identified, with 28 common in the three fractions. Among 20 most highly expressed miRNAs in each fraction, 14 were expressed in common and 11 were further shared with mammary gland tissue. The three milk fractions demonstrated a clear separation from each other using a hierarchical cluster analysis with milk fat and whey being most closely related. The miRNome correlation between milk fat and mammary gland tissue (r(mean) = 0.866) was significantly higher than the other two pairs (p < 0.01), whey/mammary gland tissue (r(mean) = 0.755) and milk cell/mammary gland tissue (r(mean) = 0.75), suggesting that milk fat could be an alternative non-invasive source of RNA in assessing miRNA activities in bovine mammary gland. Predicted target genes (1802) of 14 highly expressed miRNAs in milk fractions were enriched in fundamental cellular functions, infection, organ and tissue development. Furthermore, some miRNAs were highly enriched (FDR <0.05) in milk whey (3), cells (11) and mammary gland tissue (14) suggesting specific regulatory functions in the various fractions. In conclusion, we have obtained a comprehensive miRNA profile of the different milk fractions using high throughput sequencing. Our comparative analysis showed that miRNAs from milk fat accurately portrayed the miRNome of mammary gland tissue. Functional annotation of the top expressed miRNAs in milk confirmed their critical regulatory roles in mammary gland functions and potentially to milk recipients.
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spelling pubmed-48396142016-04-29 Comparative Analysis of the miRNome of Bovine Milk Fat, Whey and Cells Li, Ran Dudemaine, Pier-Luc Zhao, Xin Lei, Chuzhao Ibeagha-Awemu, Eveline Mengwi PLoS One Research Article Abundant miRNAs have been identified in milk and mammary gland tissues of different species. Typically, RNA in milk can be extracted from different fractions including fat, whey and cells and the mRNA transcriptome of milk could serve as an indicator of the transcriptome of mammary gland tissue. However, it has not been adequately validated if the miRNA transcriptome of any milk fraction could be representative of that of mammary gland tissue. The objectives of this study were to (1) characterize the miRNA expression spectra from three milk fractions- fat, whey and cells; (2) compare miRNome profiles of milk fractions (fat, whey and cells) with mammary gland tissue miRNome, and (3) determine which milk fraction miRNome profile could be a better representative of the miRNome profile of mammary gland tissue. Milk from four healthy Canadian Holstein cows in mid lactation was collected and fractionated. Total RNA extracted from each fraction was used for library preparation followed by small RNA sequencing. In addition, miRNA transcripts of mammary gland tissues from twelve Holstein cows in our previous study were used to compare our data. We identified 210, 200 and 249 known miRNAs from milk fat, whey and cells, respectively, with 188 universally expressed in the three fractions. In addition, 33, 31 and 36 novel miRNAs from milk fat, whey and cells were identified, with 28 common in the three fractions. Among 20 most highly expressed miRNAs in each fraction, 14 were expressed in common and 11 were further shared with mammary gland tissue. The three milk fractions demonstrated a clear separation from each other using a hierarchical cluster analysis with milk fat and whey being most closely related. The miRNome correlation between milk fat and mammary gland tissue (r(mean) = 0.866) was significantly higher than the other two pairs (p < 0.01), whey/mammary gland tissue (r(mean) = 0.755) and milk cell/mammary gland tissue (r(mean) = 0.75), suggesting that milk fat could be an alternative non-invasive source of RNA in assessing miRNA activities in bovine mammary gland. Predicted target genes (1802) of 14 highly expressed miRNAs in milk fractions were enriched in fundamental cellular functions, infection, organ and tissue development. Furthermore, some miRNAs were highly enriched (FDR <0.05) in milk whey (3), cells (11) and mammary gland tissue (14) suggesting specific regulatory functions in the various fractions. In conclusion, we have obtained a comprehensive miRNA profile of the different milk fractions using high throughput sequencing. Our comparative analysis showed that miRNAs from milk fat accurately portrayed the miRNome of mammary gland tissue. Functional annotation of the top expressed miRNAs in milk confirmed their critical regulatory roles in mammary gland functions and potentially to milk recipients. Public Library of Science 2016-04-21 /pmc/articles/PMC4839614/ /pubmed/27100870 http://dx.doi.org/10.1371/journal.pone.0154129 Text en © 2016 Li et al http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Li, Ran
Dudemaine, Pier-Luc
Zhao, Xin
Lei, Chuzhao
Ibeagha-Awemu, Eveline Mengwi
Comparative Analysis of the miRNome of Bovine Milk Fat, Whey and Cells
title Comparative Analysis of the miRNome of Bovine Milk Fat, Whey and Cells
title_full Comparative Analysis of the miRNome of Bovine Milk Fat, Whey and Cells
title_fullStr Comparative Analysis of the miRNome of Bovine Milk Fat, Whey and Cells
title_full_unstemmed Comparative Analysis of the miRNome of Bovine Milk Fat, Whey and Cells
title_short Comparative Analysis of the miRNome of Bovine Milk Fat, Whey and Cells
title_sort comparative analysis of the mirnome of bovine milk fat, whey and cells
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC4839614/
https://www.ncbi.nlm.nih.gov/pubmed/27100870
http://dx.doi.org/10.1371/journal.pone.0154129
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