Identification and characterization of miRNAs expressed in the bovine ovary

Hossain, Munir; Ghanem, Nasser; Hoelker, M.; Rings, F.; Phatsara, C.; Tholen, Ernst; Schellander, K.; Tesfaye, Dawit

doi:10.1186/1471-2164-10-443

Cited by 132 publications

(115 citation statements)

References 84 publications

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“…An increase in the levels of all of these miRNAs in large follicles was accounted for increases in mural granulosa cells rather than in COC; this was not surprising as the latter contains a very small fraction of the total cells in the follicle, and therefore microarray analyses of whole follicle tissues might have missed changes in miRNA levels in the COC. Indeed, miRNAs differentially expressed in bovine COCs, cumulus cells or oocytes, in addition to changes in miRNA expression during oocyte maturation, have been reported (Hossain et al 2009, Miles et al 2012, and they did not include any of the miRNAs identified as enriched in large healthy follicles in this study. Nonetheless, our results suggest a potential involvement of bta-miR-144, bta-miR-202, bta-miR-451, bta-miR-652, and bta-miR-873 in the regulation of mural granulosa cell function during maturation of the dominant follicle, as their expression in all cases increased in healthy follicles once they reached a diameter of 12-14 mm.…”

Section: Discussionmentioning

confidence: 86%

“…QPCR analyses confirmed that at least three of these miRNAs were also upregulated significantly in some or all of the large healthy follicle categories relative to large atretic follicles, thus identifying this set of miRNAs as very strong candidates with a role in the development of bovine dominant follicles. mir-144, mir-202, mir-451, and mir-652 were reported earlier to be expressed in the ovary (Hossain et al 2009, McBride et al 2012, Kitahara et al 2013, Schauer et al 2013, although their expression patterns within follicular tissues were not studied in detail. In this study, bta-miR-202 was restricted to the bovine gonad; moreover, its expression within the follicle was highest in granulosa cells while levels in ovarian stroma were negligible.…”

Section: Discussionmentioning

confidence: 99%

“…With a few exceptions (Carletti et al 2010, Kitahara et al 2013, most evidence on follicular roles of miRNAs has been obtained using cultured cells, particularly rodent cells, and in some cases actual changes in the expression of these miRNAs during follicle development have not been demonstrated. Indeed, although genome-wide miRNA analyses of whole ovarian tissues (Landgraf et al 2007, Ro et al 2007, Mishima et al 2008, Hossain et al 2009, Ahn et al 2010, Juanchich et al 2013 or follicular, or luteal tissues (Fiedler et al 2008, McBride et al 2012, Miles et al 2012, da Silveira et al 2012, Donadeu & Schauer 2013, Schauer et al 2013, Sohel et al 2013 have been reported in several species, detailed spatiotemporal profiles encompassing several follicle developmental stages have not. Identifying such profiles will be an important step toward understanding the functional involvement of miRNAs during specific stages of follicle development.…”

Section: Introductionmentioning

confidence: 99%

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Characterization of microRNAs differentially expressed during bovine follicle development

Sontakke¹,

Mohammed²,

McNeilly³

et al. 2014

Reproduction

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Several different miRNAs have been proposed to regulate ovarian follicle function; however, very limited information exists on the spatiotemporal patterns of miRNA expression during follicle development. The objective of this study was to identify, using microarray, miRNA profiles associated with growth and regression of dominant-size follicles in the bovine monovular ovary and to characterize their spatiotemporal distribution during development. The follicles were collected from abattoir ovaries and classified as small (4-8 mm) or large (12-17 mm); the latter were further classified as healthy or atretic based on estradiol and CYP19A1 levels. Six pools of small follicles and individual large healthy (nZ6) and large atretic (nZ5) follicles were analyzed using Exiqon's miRCURY LNA microRNA Array 6th gen, followed by qPCR validation. A total of 17 and 57 sequences were differentially expressed (greater than or equal to twofold; P!0.05) between large healthy and each of small and large atretic follicles respectively. Bovine miRNAs confirmed to be upregulated in large healthy follicles relative to small follicles (bta-miR-144, bta-miR-202, bta-miR-451, bta-miR-652, and bta-miR-873) were further characterized. Three of these miRNAs (bta-miR-144, bta-miR-202, and bta-miR-873) were also downregulated in large atretic follicles relative to large healthy follicles. Within the follicle, these miRNAs were predominantly expressed in mural granulosa cells. Further, body-wide screening revealed that bta-miR-202, but not other miRNAs, was expressed exclusively in the gonads. Finally, a total of 1359 predicted targets of the five miRNAs enriched in large healthy follicles were identified, which mapped to signaling pathways involved in follicular cell proliferation, steroidogenesis, prevention of premature luteinization, and oocyte maturation.

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Section: Discussionmentioning

confidence: 86%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

See 1 more Smart Citation

Characterization of microRNAs differentially expressed during bovine follicle development

Sontakke¹,

Mohammed²,

McNeilly³

et al. 2014

Reproduction

View full text Add to dashboard Cite

show abstract

“…F X DONADEU and others 325 ), equine follicular fluid (da Silveira et al 2012) and bovine corpora lutea have been identified using mouse-or human-based microarray or highthroughput qPCR. Some studies reported differences in miRNA expression between different ovarian or follicular compartments, including expression of miR-503, miR-224 and miR-383 predominantly in mouse granulosa cells and oocytes of mice (Lei et al 2010, Yao et al 2010a, Yin et al 2012, as well as differential expression of several dozen miRNAs in bovine ovarian cortex, cumulus cells and corpus luteum (CL; Hossain et al 2009). Further, a correlation was reported between follicular fluid and granulosa cell levels of several miRNAs in horses (da Silveira et al 2012).…”

Section: Identification and Profiling Of Mirnas In Ovarian Tissuesmentioning

confidence: 99%

“…Small RNA populations have been identified by cloningbased or next-generation sequencing of normal ovarian tissues from human (Landgraf et al 2007), mice (Ro et al 2007, Mishima et al 2008, Ahn et al 2010, pigs , cattle (Hossain et al 2009, Tripurani et al 2010, Huang et al 2011, Miles et al 2012 and sheep (McBride et al 2012). Most of those studies involved analyses on whole ovaries rather than on specific ovarian tissue components, an approach that, although very useful for comprehensive identification of miRNA sequences, provides very limited insight into their functional relevance.…”

Section: Identification and Profiling Of Mirnas In Ovarian Tissuesmentioning

confidence: 99%

Involvement of miRNAs in ovarian follicular and luteal development

Donadeu¹,

Schauer²,

Sontakke³

2012

Journal of Endocrinology

159

110

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Although much progress has been made in the genetic dissection of biological networks involved in follicular/luteal development in the mammalian ovary, the gene regulation mechanisms involved are still poorly understood. Over the last 10 years, miRNAs have emerged as master regulators of tissue growth and differentiation in animals. However, compared with other body tissues, little is still known about the functional involvement of miRNAs in the ovary. Several studies have identified miRNA populations specifically associated with the development of follicles and corpora lutea, particularly in relation to the follicular-luteal transition, and the functional involvement of some of these miRNAs has been characterised in vitro and/or in vivo. Specifically, three different miRNAs, miR-224, miR-378 and miR-383, have shown to be involved in regulating aromatase expression during follicle development. In addition, miR-21 has been identified as promoting follicular cell survival during ovulation, and pro-angiogenic miR-17-5p and let-7b were shown to be necessary for normal development of the corpus luteum. Experimental evidence for the involvement of several other miRNAs in different aspects of follicle/luteal development has also been obtained. In addition, many of these studies exemplify the challenges associated with identifying physiologically relevant targets of ovarian miRNAs. Continuous advances in this field will be considerably facilitated by progress in understanding miRNA physiology in other body systems and will eventually lead to a much better understanding of the control of follicular/luteal development. In turn, through the potential offered by miRNA diagnostics and miRNA therapeutics, this new knowledge should bring considerable benefits to reproductive medicine.

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