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Publication : High-throughput identification of Toxoplasma gondii effector proteins that target host cell transcription.

First Author  Butterworth S Year  2023
Journal  Cell Host Microbe Volume  31
Issue  10 Pages  1748-1762.e8
PubMed ID  37827122 Mgi Jnum  J:353110
Mgi Id  MGI:7548203 Doi  10.1016/j.chom.2023.09.003
Citation  Butterworth S, et al. (2023) High-throughput identification of Toxoplasma gondii effector proteins that target host cell transcription. Cell Host Microbe 31(10):1748-1762.e8
abstractText  Intracellular pathogens and other endosymbionts reprogram host cell transcription to suppress immune responses and recalibrate biosynthetic pathways. This reprogramming is critical in determining the outcome of infection or colonization. We combine pooled CRISPR knockout screening with dual host-microbe single-cell RNA sequencing, a method we term dual perturb-seq, to identify the molecular mediators of these transcriptional interactions. Applying dual perturb-seq to the intracellular pathogen Toxoplasma gondii, we are able to identify previously uncharacterized effector proteins and directly infer their function from the transcriptomic data. We show that TgGRA59 contributes to the export of other effector proteins from the parasite into the host cell and identify an effector, TgSOS1, that is necessary for sustained host STAT6 signaling and thereby contributes to parasite immune evasion and persistence. Together, this work demonstrates a tool that can be broadly adapted to interrogate host-microbe transcriptional interactions and reveal mechanisms of infection and immune evasion.
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