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An optimized method for gene knockdown in differentiating human and mouse adipocyte cultures. | LitMetric

An optimized method for gene knockdown in differentiating human and mouse adipocyte cultures.

bioRxiv

Program in Cardiovascular and Metabolic Diseases, Duke-NUS Medical School, Singapore.

Published: December 2023

AI Article Synopsis

  • Adipocyte cultures are important for studying metabolic diseases, but traditional methods for delivering siRNA to lipid-rich adipocytes don't work well, leading to challenges in research.* -
  • Alternative delivery methods like electroporation and viral systems are either too complicated, costly, or cause too much cell death, making them less favorable.* -
  • The study successfully developed a straightforward siRNA transfection protocol that works effectively on both human and mouse adipocyte cultures throughout their differentiation process, enhancing the potential for gene manipulation in these cells.*

Article Abstract

Adipocyte cultures are a mainstay of metabolic disease research, yet loss-of-function studies in differentiating adipocytes is complicated by the refractoriness of lipid-containing adipocytes to standard siRNA transfections. Alternative methods, such as electroporation or adenovirus/lentivirus-based delivery systems are complex, expensive and often accompanied with unacceptable levels of cell death. To address this problem, we have tested two commercially available siRNA delivery systems in this study using a multi-parameter optimization approach. Our results identified a uniform siRNA transfection protocol that can be applied to human and mouse adipocyte cultures throughout the time course of differentiation, beginning with pre-differentiated cells and continuing up to lipid-accumulated differentiated adipocytes. Our findings allow for efficient transfection of human and mouse adipocyte cultures using standard and readily available methodologies, and should help significantly expand the scope of gene manipulation studies in these cell types.

Download full-text PDF

Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10760114PMC
http://dx.doi.org/10.1101/2023.12.14.571780DOI Listing

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