Open this publication in new window or tab >>2020 (English)Doctoral thesis, comprehensive summary (Other academic)
Abstract [en]
The ability to profile transcriptomes and proteomes in a high-throughput fashion in single cells has truly revolutionized functional genomics, and countless functional and regulatory insights have been based on these technologies. While major applications include the discovery of new cell types and the a posteriori sorting of cell populations, studies of gene expression noise and gene co-expression have made use of this inter-cellular heterogeneity in a genuine quantitative fashion. Yet, there are still major limitations to overcome.
First, strong dynamic processes, such as cell cycle or differentiation axes, tend to overshadow more subtle underlying regulatory processes. While this has sparked the development of tools that can identify and correct these biases at large, few insights into the subtleties of gene regulation have been published thus far. The majority of studies still focus on drastic changes such as differentiation or disease. We address this issue in paper I and to a limited extend in paper II and paper III through the elimination of major confounders during experimental design. In these papers, we show that variation and covariation of miRNAs, mRNAs and proteins between individual cells of a homogeneous non-dynamic population are informative of gene regulation.
Second, while single-cell technologies are booming, with new technologies being published every day, the co-profiling of RNA and protein in the same single cells still remains a major challenge. All current technologies are limited either by protein location or throughput, or require invasive cell fixation that can compromise mRNA stability. We overcome these limitations in paper II through the combination of quantitative single-cell RNA sequencing with proximity extension assays for protein detection. Using this technology, SPARC, we show that transcription factor protein, but not transcription factor RNA, covaries with the RNA expression of its targets. We also show that translation is a major mediator of the shift in variation from the RNA to the protein level.
Third, some technologies still suffer from limited sensitivity. While, for instance, the first single-cell miRNA detection already succeeded in 2006 and the first single-cell small RNA sequencing technique was published in 2016, few insights into miRNA dynamics or function have been gained from single-cell data since. Using an optimized single-cell small RNA sequencing protocol, we quantify the miRNA transcriptome of close to 200 single cells in paper III. We show that variation and covariation can be linked to miRNA transcription and turnover. Integrating miRNA and miRNA target data from all three papers, we present evidence that the induction of variation on the RNA level and the buffering of protein expression noise are naturally occurring for many miRNAs.
In summary, we present new strategies and new protocols that overcome existing limitations in the field, and we present regulatory insights that were enabled by quantitative measurements of single-cell gene expression variation and covariation.
Place, publisher, year, edition, pages
Stockholm: Department of Molecular Biosciences, the Wenner-Gren Insitute, Stockholm University, 2020. p. 63
Keywords
Single-cell, quantitative, RNA biology, miRNA, functional genomics
National Category
Biological Sciences Bioinformatics and Computational Biology
Research subject
Molecular Bioscience
Identifiers
urn:nbn:se:su:diva-187015 (URN)978-91-7911-364-3 (ISBN)978-91-7911-365-0 (ISBN)
Public defence
2021-01-15, online via Zoom; the link will be publicly available on the department website, 09:00 (English)
Opponent
Supervisors
2020-12-212020-11-302025-02-05Bibliographically approved