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2. Single-cell multi-omic analysis of thymocyte development reveals drivers of CD4/CD8 lineage commitment

Author

Zoë Steier, Dominik A. Aylard, Laura L. McIntyre, Isabel Baldwin, Esther Jeong Yoon Kim, Lydia K. Lutes, Can Ergen, Tse-Shun Huang, Ellen A. Robey, Nir Yosef, and Aaron Streets

Subjects
Transcriptome, Thymocyte, Lineage (genetic), medicine.anatomical_structure, Mechanism (biology), Cell, medicine, Cytotoxic T cell, NFAT, Biology, CD8, Cell biology
Abstract

The development of CD4 and CD8 T cells in the thymus is critical to adaptive immunity and is widely studied as a model of lineage commitment. Recognition of self-MHCI/II by the T cell antigen receptor (TCR) determines the lineage choice, but how distinct TCR signals drive transcriptional programs of lineage commitment remains largely unknown. We applied CITE-seq to measure RNA and surface proteins in thymocytes from wild-type and lineage-restricted mice to generate a comprehensive timeline of cell state for each lineage. These analyses revealed a sequential process whereby all thymocytes initiate CD4 lineage differentiation during an initial wave of TCR signaling, followed by a second TCR signaling wave that coincides with CD8 lineage specification. CITE-seq and pharmaceutical inhibition experiments implicate a TCR/calcineurin/NFAT/GATA3 axis in driving the CD4 fate. Overall, our data suggest that multiple redundant mechanisms contribute to the accuracy and efficiency of the lineage choice.

Published
2021

4. Joint probabilistic modeling of single-cell multi-omic data with totalVI

Author

Adam Gayoso, Romain Lopez, Nir Yosef, Aaron M. Streets, Zoë Steier, Kristopher L. Nazor, and Jeffrey Regier

Subjects
Data Analysis, Technology, Computer science, Cells, Inference, Computational biology, computer.software_genre, Inbred C57BL, Biochemistry, Medical and Health Sciences, Article, Transcriptome, 03 medical and health sciences, Mice, Animals, Representation (mathematics), Molecular Biology, Cells, Cultured, 030304 developmental biology, 0303 health sciences, Computational model, Cultured, Dimensionality reduction, Search engine indexing, Probabilistic logic, Proteins, Cell Biology, Biological Sciences, High-Throughput Screening Assays, Mice, Inbred C57BL, RNA, Female, Lymph Nodes, Single-Cell Analysis, computer, Spleen, Biotechnology, Data integration, Developmental Biology
Abstract

The paired measurement of RNA and surface proteins in single cells with cellular indexing of transcriptomes and epitopes by sequencing (CITE-seq) is a promising approach to connect transcriptional variation with cell phenotypes and functions. However, combining these paired views into a unified representation of cell state is made challenging by the unique technical characteristics of each measurement. Here we present Total Variational Inference (totalVI; https://scvi-tools.org ), a framework for end-to-end joint analysis of CITE-seq data that probabilistically represents the data as a composite of biological and technical factors, including protein background and batch effects. To evaluate totalVI's performance, we profiled immune cells from murine spleen and lymph nodes with CITE-seq, measuring over 100 surface proteins. We demonstrate that totalVI provides a cohesive solution for common analysis tasks such as dimensionality reduction, the integration of datasets with different measured proteins, estimation of correlations between molecules and differential expression testing.

Published
2021

5. T cell self-reactivity during thymic development dictates the timing of positive selection

Author

James Kaminski, Ellen A. Robey, Nir Yosef, Silvia Ariotti, Zoë Steier, Laura L McIntyre, Shraddha Pandey, Ashley R Hoover, Aaron M. Streets, and Lydia K Lutes

Subjects
0301 basic medicine, Ion Channels, 0302 clinical medicine, Gene expression, Biology (General), Thymocytes, Chemistry, General Neuroscience, Cell Differentiation, General Medicine, Cell biology, Thymocyte, medicine.anatomical_structure, Phenotype, Self Tolerance, Medicine, TCR, Signal Transduction, QH301-705.5, Science, T cell, Receptors, Antigen, T-Cell, Mice, Transgenic, Thymus Gland, Biology, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Downregulation and upregulation, positive selection, medicine, Animals, Cell Lineage, Gene, Ion channel, General Immunology and Microbiology, Mechanism (biology), Positive selection, T-cell receptor, Histocompatibility Antigens Class I, thymocyte, Mice, Inbred C57BL, Kinetics, 030104 developmental biology, Gene Expression Regulation, self-reactivity, Transcriptome, Developmental biology, Function (biology), 030217 neurology & neurosurgery
Abstract

Functional tuning of T cells based on their degree of self-reactivity is established during positive selection in the thymus, although how positive selection differs for thymocytes with relatively low versus high self-reactivity is unclear. In addition, preselection thymocytes are highly sensitive to low-affinity ligands, but the mechanism underlying their enhanced TCR sensitivity is not fully understood. Here we show that murine thymocytes with low self-reactivity experience briefer TCR signals and complete positive selection more slowly than those with high self-reactivity. Additionally, we provide evidence that cells with low self-reactivity retain a preselection gene expression signature as they mature, including genes previously implicated in modulating TCR sensitivity and a novel group of ion channel genes. Our results imply that thymocytes with low self-reactivity down-regulate TCR sensitivity more slowly during positive selection, and suggest that modulation of membrane ion channel function may play a role in regulating TCR tuning throughout development.Impact StatementDeveloping T cells whose TCRs have relatively low reactivity experience very brief TCR signaling events, delayed positive selection, and do not fully down regulate their TCR sensitivity as they mature.

Published
2020

6. Joint probabilistic modeling of paired transcriptome and proteome measurements in single cells

Author

Adam Gayoso, Kristopher L. Nazor, Aaron M. Streets, Nir Yosef, Zoë Steier, Jeffrey Regier, and Romain Lopez

Subjects
0303 health sciences, Computer science, Cell, Probabilistic logic, RNA, Computational biology, Transcriptome, 03 medical and health sciences, 0302 clinical medicine, medicine.anatomical_structure, Proteome, medicine, Molecule, Probabilistic analysis of algorithms, Cluster analysis, Surface protein, 030304 developmental biology, 030215 immunology
Abstract

The paired measurement of RNA and surface protein abundance in single cells with CITE-seq is a promising approach to connect transcriptional variation with cell phenotypes and functions. However, each data modality exhibits unique technical biases, making it challenging to conduct a joint analysis and combine these two views into a unified representation of cell state. Here we present Total Variational Inference (totalVI), a framework for the joint probabilistic analysis of paired RNA and protein data from single cells. totalVI probabilistically represents the data as a composite of biological and technical factors such as limited sensitivity of the RNA data, background in the protein data, and batch effects. To evaluate totalVI, we performed CITE-seq on immune cells from murine spleen and lymph nodes with biological replicates and with different antibody panels measuring over 100 surface proteins. With this dataset, we demonstrate that totalVI provides a cohesive solution for common analysis tasks like the integration of datasets with matched or unmatched protein panels, dimensionality reduction, clustering, evaluation of correlations between molecules, and differential expression testing. totalVI enables scalable, end-to-end analysis of paired RNA and protein data from single cells and is available as open-source software.

Published
2020

7. CXCR3 regulates stem and proliferative CD8+ T cells during chronic infection by promoting interactions with DCs in splenic bridging channels

Author

Derek J. Bangs, Alexandra Tsitsiklis, Zoë Steier, Shiao Wei Chan, James Kaminski, Aaron Streets, Nir Yosef, and Ellen A. Robey

Subjects
white pulp, Receptors, CXCR3, Medical Physiology, Toxoplasma gondii, CD8-Positive T-Lymphocytes, General Biochemistry, Genetics and Molecular Biology, Mice, stomatognathic system, Receptors, 2.1 Biological and endogenous factors, Animals, Aetiology, CXCR3, Animal, CXCL10, bridging channel, Prevention, red pulp, Cell Differentiation, Dendritic Cells, Lymphoid Progenitor Cells, chronic infection, Stem Cell Research, Foodborne Illness, CD8+ T cell differentiation, stomatognathic diseases, cDC-2s, Infectious Diseases, Emerging Infectious Diseases, Toxoplasmosis, Animal, CXCL9, Persistent Infection, Biochemistry and Cell Biology, Infection, Toxoplasmosis, Spleen
Abstract

Production of effector CD8+ Tcells during persistent infection requires a stable pool of stem-like cells that can give rise to effector cells via a proliferative intermediate population. In infection models marked by Tcell exhaustion, this process can be transiently induced by checkpoint blockade but occurs spontaneously in mice chronically infected with the protozoan intracellular parasite Toxoplasma gondii. We observe distinct locations for parasite-specific Tcell subsets, implying a link between differentiation and anatomical niches in the spleen. Loss of the chemokine receptor CXCR3 on Tcells does not prevent white pulp-to-red pulp migration but reduces interactions with CXCR3 ligand-producing dendritic cells (DCs) and impairs memory-to-intermediate transition, leading to a buildup of memory Tcells in the red pulp. Thus, CXCR3 increases Tcell exposure to differentiation-inducing signals during red pulp migration, providing a dynamic mechanism for modulating effector differentiation in response to environmental signals.

Published
2022

8. Flucytosine Antagonism of Azole Activity versus Candida glabrata: Role of Transcription Factor Pdr1 and Multidrug Transporter Cdr1

Author

Santosh K. Katiyar, Geoffrey Toner, Thomas D. Edlind, John-Paul Vermitsky, Zoë Steier, and Scott E. Gygax

Subjects
Antifungal Agents, Flucytosine, Candida glabrata, Biology, Pharmacology, Microbiology, Fungal Proteins, Downregulation and upregulation, Mechanisms of Resistance, Drug Resistance, Fungal, Gene Expression Regulation, Fungal, medicine, Pharmacology (medical), Fluconazole, Drug Antagonism, chemistry.chemical_classification, Fungal protein, biology.organism_classification, Mitochondria, Infectious Diseases, chemistry, Azole, ATP-Binding Cassette Transporters, Drug Therapy, Combination, Antagonism, Transcription Factors, medicine.drug
Abstract

Infections with the opportunistic yeast Candida glabrata have increased dramatically in recent years. Antifungal therapy of yeast infections commonly employs azoles, such as fluconazole (FLC), but C. glabrata frequently develops resistance to these inhibitors of ergosterol biosynthesis. The pyrimidine analog flucytosine (5-fluorocytosine [5FC]) is highly active versus C. glabrata but is now rarely used clinically due to similar concerns over resistance and, a related concern, the toxicity associated with high doses used to counter resistance. Azole-5FC combination therapy would potentially address these concerns; however, previous studies suggest that 5FC may antagonize azole activity versus C. glabrata . Here, we report that 5FC at subinhibitory concentrations antagonized the activity of FLC 4- to 16-fold versus 8 of 8 C. glabrata isolates tested. 5FC antagonized the activity of other azoles similarly but had only indifferent effects in combination with unrelated antifungals. Since azole resistance in C. glabrata results from transcription factor Pdr1-dependent upregulation of the multidrug transporter gene CDR1 , we reasoned that 5FC antagonism might be similarly mediated. Indeed, 5FC-FLC antagonism was abrogated in pdr1 Δ and cdr1 Δ strains. In further support of this hypothesis, 5FC exposure induced CDR1 expression 6-fold, and this upregulation was Pdr1 dependent. In contrast to azoles, 5FC is not a Cdr1 substrate and so its activation of Pdr1 was unexpected. We observed, however, that 5FC exposure readily induced petite mutants, which exhibit Pdr1-dependent CDR1 upregulation. Thus, mitochondrial dysfunction resulting in Pdr1 activation is the likely basis for 5FC antagonism of azole activity versus C. glabrata .

Published
2013

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