In vivo CRISPR screens reveal a HIF-1α-mTOR-network regulates T follicular helper versus Th1 cells.
Bonnie HuangJames D PhelanSilvia PreiteJulio Gomez-RodriguezKristoffer Haurum JohansenHirofumi ShibataArthur L ShafferQin XuBrendan JeffreyMartha KirbyStacie AndersonYandan YangSelamawit GossaDorian B McGavernLouis M StaudtPamela L SchwartzbergPublished in: Nature communications (2022)
T follicular helper (Tfh) cells provide signals to initiate and maintain the germinal center (GC) reaction and are crucial for the generation of robust, long-lived antibody responses, but how the GC microenvironment affects Tfh cells is not well understood. Here we develop an in vivo T cell-intrinsic CRISPR-knockout screen to evaluate Tfh and Th1 cells in an acute viral infection model to identify regulators of Tfh cells in their physiological setting. Using a screen of druggable-targets, alongside genetic, transcriptomic and cellular analyses, we identify a function of HIF-1α in suppressing mTORC1-mediated and Myc-related pathways, and provide evidence that VHL-mediated degradation of HIF-1α is required for Tfh development; an expanded in vivo CRISPR screen reveals multiple components of these pathways that regulate Tfh versus Th1 cells, including signaling molecules, cell-cycle regulators, nutrient transporters, metabolic enzymes and autophagy mediators. Collectively, our data serve as a resource for studying Tfh versus Th1 decisions, and implicate the VHL-HIF-1α axis in fine-tuning Tfh generation.
Keyphrases
- induced apoptosis
- cell cycle arrest
- genome wide
- cell cycle
- endoplasmic reticulum stress
- signaling pathway
- cell death
- cell proliferation
- high throughput
- oxidative stress
- crispr cas
- machine learning
- liver failure
- transcription factor
- endothelial cells
- dna methylation
- stem cells
- single cell
- immune response
- high resolution
- copy number
- genome editing
- artificial intelligence
- liquid chromatography
- gas chromatography