AI Article Synopsis

  • The snATAC + snRNA platform allows researchers to analyze open chromatin and gene expression at a single-cell level, emphasizing the importance of high-quality nuclei isolation.
  • Different nuclei isolation methods were tested on human tissue samples, particularly peripheral blood mononuclear cells and ovarian cancer tissues, revealing that NP-40 detergent-based isolation provided superior sequencing results compared to collagenase tissue dissociation.
  • The study confirmed that both frozen and fresh sample preparations yield high-quality data, and it highlighted the effectiveness of using both scRNA and snRNA for accurate cell type identification in multiomic assays.

Article Abstract

The snATAC + snRNA platform allows epigenomic profiling of open chromatin and gene expression with single-cell resolution. The most critical assay step is to isolate high-quality nuclei to proceed with droplet-base single nuclei isolation and barcoding. With the increasing popularity of multiomic profiling in various fields, there is a need for optimized and reliable nuclei isolation methods, mainly for human tissue samples. Herein we compared different nuclei isolation methods for cell suspensions, such as peripheral blood mononuclear cells (PBMC, = 18) and a solid tumor type, ovarian cancer (OC, = 18), derived from debulking surgery. Nuclei morphology and sequencing output parameters were used to evaluate the quality of preparation. Our results show that NP-40 detergent-based nuclei isolation yields better sequencing results than collagenase tissue dissociation for OC, significantly impacting cell type identification and analysis. Given the utility of applying such techniques to frozen samples, we also tested frozen preparation and digestion ( = 6). A paired comparison between frozen and fresh samples validated the quality of both specimens. Finally, we demonstrate the reproducibility of scRNA and snATAC + snRNA platform, by comparing the gene expression profiling of PBMC. Our results highlight how the choice of nuclei isolation methods is critical for obtaining quality data in multiomic assays. It also shows that the measurement of expression between scRNA and snRNA is comparable and effective for cell type identification.

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Source
http://www.ncbi.nlm.nih.gov/pmc/articles/PMC10297939PMC
http://dx.doi.org/10.3390/genes14061245DOI Listing

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