PT  - JOURNAL ARTICLE
AU  - Daniel Conde
AU  - Paolo M. Triozzi
AU  - Kelly M. Balmant
AU  - Andria L. Doty
AU  - Mariza Miranda
AU  - Anthony Boullosa
AU  - Henry W. Schmidt
AU  - Wendell J. Pereira
AU  - Christopher Dervinis
AU  - Matias Kirst
TI  - A robust method of nuclei isolation for single-cell RNA sequencing of solid tissues from the plant genus &lt;em&gt;Populus&lt;/em&gt;
AID  - 10.1101/2021.02.11.430521
DP  - 2021 Jan 01
TA  - bioRxiv
PG  - 2021.02.11.430521
4099  - http://biorxiv.org/content/early/2021/02/12/2021.02.11.430521.short
4100  - http://biorxiv.org/content/early/2021/02/12/2021.02.11.430521.full
AB  - Single-cell transcriptome analysis has been extensively applied in humans and animal models to uncover gene expression heterogeneity between the different cell types of a tissue or an organ. It demonstrated its capability to discover the key regulatory elements that determine cell fate during developmental programs such as brain or heart development. Single-cell analysis requires the isolation and labeling of the messenger RNA (mRNA) derived from each cell. These challenges were primarily addressed in mammals by developing microfluidic-based approaches. For plant species whose cells contain cell walls, these approaches have generally required the generation of isolated protoplasts. Many plant tissues’ secondary cell wall hinders enzymatic digestion required for individual protoplast isolation, resulting in an unequal representation of cell types in a protoplast population. This limitation is especially critical for cell types located in the inner layers of a tissue or the inner tissues of an organ. Consequently, single-cell RNA sequencing (scRNA-seq) studies using microfluidic approaches in plants have mainly been restricted to Arabidopsis roots, for which well-established procedures of protoplast isolation are available. Here we present a simple alternative approach to generating high-quality protoplasts from plant tissue by characterizing the mRNA extracted from individual nuclei instead of whole cells. We developed the protocol using two different plant materials with varying cellular complexity levels and cell-wall structure, Populus shoot apices, and more lignified stems. Using the 10× Genomics Chromium technology, we show that this procedure results in intact mRNA isolation and limited leakage, with a broad representation of individual cell transcriptomes.Competing Interest StatementThe authors have declared no competing interest.