[HTML][HTML] Protocol for primary mouse hepatocyte isolation
M Charni-Natan, I Goldstein - STAR protocols, 2020 - Elsevier
M Charni-Natan, I Goldstein
STAR protocols, 2020•ElsevierPrimary hepatocytes are a vital tool in various biomedical research disciplines, serving as an
ex vivo model for liver physiology. Obtaining high yields of viable primary mouse
hepatocytes is technically challenging, limiting their use. Here, we present an improved
protocol based on the classic two-step collagenase perfusion technique. The liver is washed
by perfusion, hepatocytes are dissociated by collagenase, separated from other cells, and
cultured. This protocol was optimized to significantly reduce procedure duration and improve …
ex vivo model for liver physiology. Obtaining high yields of viable primary mouse
hepatocytes is technically challenging, limiting their use. Here, we present an improved
protocol based on the classic two-step collagenase perfusion technique. The liver is washed
by perfusion, hepatocytes are dissociated by collagenase, separated from other cells, and
cultured. This protocol was optimized to significantly reduce procedure duration and improve …
Summary
Primary hepatocytes are a vital tool in various biomedical research disciplines, serving as an ex vivo model for liver physiology. Obtaining high yields of viable primary mouse hepatocytes is technically challenging, limiting their use. Here, we present an improved protocol based on the classic two-step collagenase perfusion technique. The liver is washed by perfusion, hepatocytes are dissociated by collagenase, separated from other cells, and cultured. This protocol was optimized to significantly reduce procedure duration and improve hepatocyte yield and viability.
Elsevier