[HTML][HTML] Preparing highly viable single-cell suspensions from mouse pancreatic islets for single-cell RNA sequencing
H Lee, F Engin - STAR protocols, 2020 - Elsevier
H Lee, F Engin
STAR protocols, 2020•ElsevierPancreatic islets consist of several cell types, including alpha, beta, delta, epsilon, and PP
cells. Due to cellular heterogeneity, it is challenging to interpret whole-islet transcriptome
data. Single-cell transcriptomics offers a powerful method for investigating gene expression
at the single-cell level and identifying cellular heterogeneity and subpopulations. Here, we
describe a protocol for mouse pancreatic islet isolation, culturing, and dissociation into a
single-cell suspension. This protocol yields highly viable cells for successful library …
cells. Due to cellular heterogeneity, it is challenging to interpret whole-islet transcriptome
data. Single-cell transcriptomics offers a powerful method for investigating gene expression
at the single-cell level and identifying cellular heterogeneity and subpopulations. Here, we
describe a protocol for mouse pancreatic islet isolation, culturing, and dissociation into a
single-cell suspension. This protocol yields highly viable cells for successful library …
Summary
Pancreatic islets consist of several cell types, including alpha, beta, delta, epsilon, and PP cells. Due to cellular heterogeneity, it is challenging to interpret whole-islet transcriptome data. Single-cell transcriptomics offers a powerful method for investigating gene expression at the single-cell level and identifying cellular heterogeneity and subpopulations. Here, we describe a protocol for mouse pancreatic islet isolation, culturing, and dissociation into a single-cell suspension. This protocol yields highly viable cells for successful library preparation and single-cell RNA sequencing.
For complete details on the use and execution of this protocol, please refer to Lee et al. (2020).
Elsevier