Rapid generation of functional nanovesicles from human trophectodermal cells for embryo attachment and outgrowth

Author:

Poh Qi Hui123ORCID,Rai Alin134ORCID,Pangestu Mulyoto5ORCID,Salamonsen Lois A.6ORCID,Greening David W.12347ORCID

Affiliation:

1. Baker Heart and Diabetes Institute Molecular Proteomics Melbourne Victoria Australia

2. Department of Biochemistry and Chemistry School of Agriculture, Biomedicine and Environment La Trobe University Bundoora Victoria Australia

3. Department of Cardiovascular Research, Translation and Implementation La Trobe University Melbourne Victoria Australia

4. Central Clinical School Monash University Melbourne Victoria Australia

5. Education Program in Reproduction and Development (EPRD) Department of Obstetrics and Gynaecology Monash Clinical School Monash University Clayton Victoria Australia

6. Hudson Institute of Medical Research and Monash University Clayton Victoria Australia

7. Baker Department of Cardiometabolic Health University of Melbourne Melbourne Victoria Australia

Abstract

AbstractExtracellular vesicles (EVs) are important mediators of embryo attachment and outgrowth critical for successful implantation. While EVs have garnered immense interest in their therapeutic potential in assisted reproductive technology by improving implantation success, their large‐scale generation remains a major challenge. Here, we report a rapid and scalable production of nanovesicles (NVs) directly from human trophectoderm cells (hTSCs) via serial mechanical extrusion of cells; these NVs can be generated in approximately 6 h with a 20‐fold higher yield than EVs isolated from culture medium of the same number of cells. NVs display similar biophysical traits (morphologically intact, spherical, 90–130 nm) to EVs, and are laden with hallmark players of implantation that include cell‐matrix adhesion and extracellular matrix organisation proteins (ITGA2/V, ITGB1, MFGE8) and antioxidative regulators (PRDX1, SOD2). Functionally, NVs are readily taken up by low‐receptive endometrial HEC1A cells and reprogram their proteome towards a receptive phenotype that support hTSC spheroid attachment. Moreover, a single dose treatment with NVs significantly enhanced adhesion and spreading of mouse embryo trophoblast on fibronectin matrix. Thus, we demonstrate the functional potential of NVs in enhancing embryo implantation and highlight their rapid and scalable generation, amenable to clinical utility.

Funder

National Health and Medical Research Council

Publisher

Wiley

Subject

Molecular Biology,Biochemistry

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