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Optimization of mouse kidney digestion protocols for single-cell applications

journal contribution
posted on 2025-03-05, 00:27 authored by Jake RobertsonJake Robertson, Henry DiepHenry Diep, Ruvantha PintoRuvantha Pinto, Christopher SobeyChristopher Sobey, Grant DrummondGrant Drummond, Antony VinhAntony Vinh, Maria JelinicMaria Jelinic

Abstract:

Single-cell technologies such as flow cytometry and single-cell RNA sequencing have allowed for comprehensive characterization of the kidney cellulome. However, there is a disparity in the various protocols for preparing kidney single-cell suspensions. We aimed to address this limitation by characterizing kidney cellular heterogeneity using three previously published single-cell preparation protocols. Single-cell suspensions were prepared from male and female C57BL/6 kidneys using the following kidney tissue dissociation protocols: a scRNAseq protocol (P1), a multi-tissue digestion kit from Miltenyi Biotec (P2), and a protocol established in our laboratory (P3). Following dissociation, flow cytometry was used to identify known major cell types including leukocytes (myeloid and lymphoid), vascular cells (smooth muscle and endothelial), nephron epithelial cells (intercalating, principal, proximal, and distal tubule cells), podocytes, and fibroblasts. Of the protocols tested, P2 yielded significantly less leukocytes and type B intercalating cells compared with the other techniques. P1 and P3 produced similar yields for most cell types; however, endothelial and myeloid-derived cells were significantly enriched using P1. Significant sex differences were detected in only two cell types: granulocytes (increased in males) and smooth muscle cells (increased in females). Future single-cell studies that aim to enrich specific kidney cell types may benefit from this comparative analysis. NEW & NOTEWORTHY This study is the first to evaluate published single-cell suspension preparation protocols and their ability to produce high-quality cellular yields from the mouse kidney. Three single-cell digestion protocols were compared and each produced significant differences in kidney cellular heterogeneity. These findings highlight the importance of the digestion protocol when using single-cell technologies. This study may help future single-cell science research by guiding researchers to choose protocols that enrich certain cell types of interest. flow cytometry; renal; single-cell RNA sequencing; tissue dissociation.

Funding

This work was funded by Jack Brockhoff Foundation Fellowship ID4519 (to M.J.), a Diabetes Australia Research Program General Grant (to M.J., A.V., and G.R.D.), and NHMRC Ideas Grant GNT2020452 (to G.R.D., A.V., and M.J.). M.J. was supported by joint NHMRC and NHF Postdoctoral Fellowships GNT1146314 and 101943. J.N.R. was supported by an Australian Research Training Scholarship and a Defence Science Institute Research Higher Degree Student Grant.

History

Publication Date

2024-07-01

Journal

Physiological Genomics

Volume

56

Issue

7

Pagination

14p. (p. 469-482)

Publisher

American Physiological Society

ISSN

1094-8341

Rights Statement

Copyright © 2024 The Authors. Licensed under Creative Commons Attribution CC-BY 4.0

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    Keywords

    flow cytometryrenalsingle-cell RNA sequencingtissue dissociation

    Licence

    CC BY 4.0

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