Optimization of microRNA Acquirement from Seminal Plasma and Identification of Diminished Seminal microRNA-34b as Indicator of Low Semen Concentration

Michael Eikmans; Jacqueline D H Anholts; Laura Blijleven; Tess Meuleman; Els van Beelen; Marie-Louise P van der Hoorn; Frans H J Claas

doi:10.3390/ijms21114089

Optimization of microRNA Acquirement from Seminal Plasma and Identification of Diminished Seminal microRNA-34b as Indicator of Low Semen Concentration

Int J Mol Sci. 2020 Jun 8;21(11):4089. doi: 10.3390/ijms21114089.

Authors

Michael Eikmans¹, Jacqueline D H Anholts¹, Laura Blijleven¹, Tess Meuleman², Els van Beelen¹, Marie-Louise P van der Hoorn³, Frans H J Claas¹

Affiliations

¹ Department of Immunohematology, Leiden University Medical Center, 2333 ZA Leiden, The Netherlands.
² Department of Gynecology and Obstetrics, Radboud University Medical Center, 6525 GA Nijmegen, The Netherlands.
³ Department of Gynecology and Obstetrics, Leiden University Medical Center, 2333 ZA Leiden, The Netherlands.

Abstract

About 10-15% of couples who want to conceive suffer from subfertility, while in 30% of these cases, a male factor plays a role. Levels of particular microRNAs in seminal plasma, including those involved in spermatogenesis, may serve as an indicative parameter for subfertility. We first optimized a protocol for acquiring microRNAs from seminal plasma. Next, using a test-validation strategy in a male cohort, we aimed to identify microRNAs of which the levels are related to semen motility and concentration. By qPCR, 742 microRNAs were profiled in three normozoospermic samples, three seminal samples with a low semen motility (asthenozoospermia), and three with a low semen concentration (oligozoospermia). MicroRNAs showing significant differences between groups were further validated in a second cohort consisting of 40 samples with normozoospermia (control group), 47 samples with asthenozoospermia, and 19 samples with oligozoospermia (of which 74% also low motility). Highest microRNA yields were obtained with the Biofluids RNA extraction kit, with inclusion of MS2 RNA carrier and proteinase K treatment to the protocol, and when 50 µL of seminal plasma was used as input. Exosome isolation prior to RNA extraction did not lead to enhanced yields. In the test cohort, 236 microRNAs could be detected, of which 54 microRNAs showed a difference between groups. Five microRNAs were analyzed in the validation cohort. MiR-34b-5p levels in the control group were significantly higher compared to the asthenozoospermia group (p < 0.05) and compared to the oligozoospermia group (p < 0.001). We optimized microRNA acquirement from seminal plasma and identified microRNA levels in relation to semen concentration and motility. As recent human and mouse studies show that the miR-34 family is a marker of low semen concentration and is crucial in spermatogenesis, seminal plasma miR-34b-5p may represent a suitable candidate to study further as a marker of male subfertility.

Keywords: asthenozoospermia; microRNA; oligozoospermia; optimization; semen; seminal plasma.

MeSH terms

Asthenozoospermia / diagnosis
Asthenozoospermia / genetics
Biomarkers
Computational Biology / methods
Gene Expression Profiling
Humans
Male
MicroRNAs / genetics*
Oligospermia / diagnosis
Oligospermia / genetics
Prognosis
Reproducibility of Results
Semen*
Sperm Count*
Spermatogenesis
Transcriptome

Substances

Biomarkers
MicroRNAs