Objective: To evaluate the feasibility of stem cell isolation from falciform fat harvested via laparoscopic morcellation.

Study Design: Pilot study.

Animals: Eleven client-owned dogs.

Methods: Falciform was harvested traditionally via laparotomy and laparoscopically via tissue morcellation. Harvested tissue was processed with a commercially available adipose tissue dissociation kit to obtain a stromal vascular fraction (SVF). Cells were subsequently labeled for CD90, CD45, and CD44 cell surface antigens by using magnetic-activated cell sorting (MACS) and fluorescence-activated cell sorting flow cytometry. CD90 cells were quantitated, and their viability was assessed with a hemocytometer and a trypan blue exclusion test of cell viability.

Results: No perioperative complications occurred in dogs undergoing laparoscopic morcellation. Laparoscopically and traditionally harvested samples yielded an average of 0.39 (±0.1) × 10 and 0.33 (±0.1) × 10 CD90 cells, respectively, per 10 million SVF cells. CD90 cell viability after MACS was 89% (±11%) for morcellated and 86% (±7%) for traditionally harvested samples. Neither CD90 cell quantity nor viability was different between samples obtained via traditional laparotomy vs laparoscopic morcellation (P = .38 and P = .63, respectively). Populations of CD90 cells isolated with each harvest technique had similar CD44 and CD45 expression profiles.

Conclusion: Viable populations of CD90 cells with similar CD44/CD45 expression profiles were isolated from laparoscopically morcellated and traditionally harvested falciform tissue. No appreciable morbidity was associated with laparoscopic falciform morcellation.

Clinical Significance: Laparoscopic morcellation is a safe and effective minimally invasive approach to falciform tissue harvest for adipose-derived mesenchymal stem cell isolation.

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http://dx.doi.org/10.1111/vsu.13267DOI Listing

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