Frontiers in Molecular Neuroscience (Oct 2018)

Assessing Transcriptome Quality in Patch-Seq Datasets

  • Shreejoy J. Tripathy,
  • Shreejoy J. Tripathy,
  • Lilah Toker,
  • Lilah Toker,
  • Claire Bomkamp,
  • B. Ogan Mancarci,
  • B. Ogan Mancarci,
  • Manuel Belmadani,
  • Manuel Belmadani,
  • Paul Pavlidis,
  • Paul Pavlidis

DOI
https://doi.org/10.3389/fnmol.2018.00363
Journal volume & issue
Vol. 11

Abstract

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Patch-seq, combining patch-clamp electrophysiology with single-cell RNA-sequencing (scRNAseq), enables unprecedented access to a neuron's transcriptomic, electrophysiological, and morphological features. Here, we present a re-analysis of five patch-seq datasets, representing cells from ex vivo mouse brain slices and in vitro human stem-cell derived neurons. Our objective was to develop simple criteria to assess the quality of patch-seq derived single-cell transcriptomes. We evaluated patch-seq transcriptomes for the expression of marker genes of multiple cell types, benchmarking these against analogous profiles from cellular-dissociation based scRNAseq. We found an increased likelihood of off-target cell-type mRNA contamination in patch-seq cells from acute brain slices, likely due to the passage of the patch-pipette through the processes of adjacent cells. We also observed that patch-seq samples varied considerably in the amount of mRNA that could be extracted from each cell, strongly biasing the numbers of detectable genes. We developed a marker gene-based approach for scoring single-cell transcriptome quality post-hoc. Incorporating our quality metrics into downstream analyses improved the correspondence between gene expression and electrophysiological features. Our analysis suggests that technical confounds likely limit the interpretability of patch-seq based single-cell transcriptomes. However, we provide concrete recommendations for quality control steps that can be performed prior to costly RNA-sequencing to optimize the yield of high-quality samples.

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