Effects of epinephrine, lidocaine, and prilocaine on viability and differentiation capacity of human adipose stem cells

Vincent G J Guillaume; Laura S Lanckohr; Ella F Lippold; Justus P Beier; Tim Ruhl

doi:10.1016/j.bjps.2023.10.104

Effects of epinephrine, lidocaine, and prilocaine on viability and differentiation capacity of human adipose stem cells

J Plast Reconstr Aesthet Surg. 2023 Dec:87:408-415. doi: 10.1016/j.bjps.2023.10.104. Epub 2023 Oct 20.

Authors

Vincent G J Guillaume¹, Laura S Lanckohr², Ella F Lippold², Justus P Beier², Tim Ruhl²

Affiliations

¹ Department of Plastic Surgery, Hand Surgery, Burn Center, University Hospital RWTH Aachen, Pauwelsstraße 30, 52074 Aachen, NRW, Germany. Electronic address: vguillaume@ukaachen.de.
² Department of Plastic Surgery, Hand Surgery, Burn Center, University Hospital RWTH Aachen, Pauwelsstraße 30, 52074 Aachen, NRW, Germany.

PMID: 37939646
DOI: 10.1016/j.bjps.2023.10.104

Abstract

Introduction: Local anesthetics (LAs) are routinely administered in plastic and reconstructive surgery, e.g., as tumescent anesthesia adjunct in liposuction. Historically, these substances were assumed to act cytotoxically. Thus, the application of LA was avoided when handling adipose stem cells (ASCs). We recently determined that most LAs are not cytotoxic when ASCs are exposed to concentrations used for tumescent liposuction. However, there is limited information when combining LA with epinephrine and about the effects of prilocaine on ASCs.

Methods: We analyzed the effects of prilocaine or lidocaine in co-exposure with epinephrine on the viability of primary human ASCs, i.e., proliferation, metabolic activity, and cytotoxicity, using crystal violet-staining, PrestoBlue®-, and WST-1 assay. We quantified the impact of short-term incubation of lidocaine and epinephrine on the differentiation of ASCs into the adipogenic, chondrogenic, and osteogenic lineage.

Results: After 2 h, prilocaine (10 mM) significantly reduced metabolic activity and cell numbers, whereas lidocaine only inhibited metabolic activity. After 6 h, prilocaine (10 mM) and lidocaine significantly decreased metabolic activity as well as cell numbers. The application of high concentrations of epinephrine did not affect cell numbers but diminished metabolic activity. Combining lidocaine with epinephrine had no additional cytotoxic effect. Differentiation into the chondrogenic lineage was significantly inhibited by epinephrine.

Conclusions: Deducing from our data, neither lidocaine combined with epinephrine nor prilocaine has a cytotoxic impact on ASCs in vitro at concentrations equivalent to those in tumescent anesthesia and has no long-lasting effect on the differentiation capacity of ASCs into the osteogenic and adipogenic lineage.

Keywords: ASCs; Catecholamines; Cytotoxicity; Fat grafting; Lipotransfer; Local anesthetics.

MeSH terms

Anesthesia, Local
Anesthetics, Local / pharmacology
Cell Differentiation
Epinephrine / pharmacology
Humans
Lidocaine* / pharmacology
Prilocaine* / pharmacology
Stem Cells

Substances

Lidocaine
Prilocaine
Anesthetics, Local
Epinephrine