Immortalized mouse caput epididymal epithelial (mECap18) cell line recapitulates the in‐vivo environment

Author:

Mulhall Jess E.12,Trigg Natalie A.34,Bernstein Ilana R.12,Anderson Amanda L.12,Murray Heather C.56ORCID,Sipilä Petra7,Lord Tessa12,Schjenken John E.12,Nixon Brett12ORCID,Skerrett‐Byrne David A.12ORCID

Affiliation:

1. Priority Research Centre for Reproductive Science School of Environmental and Life Sciences, College of Engineering, Science and Environment The University of Newcastle Callaghan New South Wales Australia

2. Infertility and Reproduction Research Program Hunter Medical Research Institute New Lambton New South Wales Australia

3. Division of Neonatology Children's Hospital of Philadelphia Philadelphia Pennsylvania USA

4. Departments of Genetics and Pediatrics ‐ Penn Epigenetics Institute Institute of Regenerative Medicine and Center for Research on Reproduction and Women's Health University of Pennsylvania Perelman School of Medicine Philadelphia Pennsylvania USA

5. School of Biomedical Sciences and Pharmacy, College of Health, Medicine and Wellbeing The University of Newcastle New South Wales New South Wales Australia

6. Precision Medicine Research Program Hunter Medical Research Institute Newcastle New South Wales Australia

7. Institute of Biomedicine Research Centre for Integrative Physiology and Pharmacology and Turku Center for Disease Modeling University of Turku Turku Varsinais‐Suomi Finland

Abstract

AbstractResiding between the testes and the vas deferens, the epididymis is a highly convoluted tubule whose unique luminal microenvironment is crucial for the functional maturation of spermatozoa. This microenvironment is created by the combined secretory and resorptive activity of the lining epididymal epithelium, including the release of extracellular vesicles (epididymosomes), which encapsulate fertility modulating proteins and a myriad of small non‐coding RNAs (sncRNAs) that are destined for delivery to recipient sperm cells. To enable investigation of this intercellular communication nexus, we have previously developed an immortalized mouse caput epididymal epithelial cell line (mECap18). Here, we describe the application of label‐free mass spectrometry to characterize the mECap18 cell proteome and compare this to the proteome of native mouse caput epididymal epithelial cells. We report the identification of 5,313 mECap18 proteins, as many as 75.8% of which were also identified in caput epithelial cells wherein they mapped to broadly similar protein classification groupings. Furthermore, key pathways associated with protein synthesis (e.g., EIF2 signaling) and cellular protection in the male reproductive tract (e.g., sirtuin signaling) were enriched in both proteomes. This comparison supports the utility of the mECap18 cell line as a tractable in‐vitro model for studying caput epididymal epithelial cell function.

Funder

Australian Education International, Australian Government

National Health and Medical Research Council

Publisher

Wiley

Subject

Molecular Biology,Biochemistry

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