Genome-wide CRISPR screens for Shiga toxins and ricin reveal Golgi proteins critical for glycosylation

Tian, Songhai; Muneeruddin, Khaja; Choi, Mei Yuk; Tao, Liang; Bhuiyan, Robiul H.; Ohmi, Yuhsuke; Furukawa, Koichi; Boland, Sebastian; Shaffer, Scott A.; Adam, Rosalyn M.; Dong, Min

doi:10.1371/journal.pbio.2006951

Cited by 72 publications

(102 citation statements)

References 60 publications

(83 reference statements)

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“…1B). LAPTM4A and TM9SF2, which have been correlated with Shiga toxin resistance (25)(26)(27), were also found to be highly enriched and among the 20 top-ranking genes in our genetic screen. Surprisingly, AHR, a transcription factor with broad physiological functions (14)(15)(16)(17)(18)(19), also showed high enrichment comparable with that observed for the SL biosynthetic genes (Fig.…”

Section: Genome-wide Crispr/cas9 Screen For Positive Regulators Of Slmentioning

confidence: 66%

“…Because the level of cell-surface Gb3 on HeLa cells correlates with their sensitivity to the toxin (23,24), we reasoned that selection of Shiga toxin-resistant HeLa cells after transduction of a genome-scale knockout (KO) library could yield not only the biosynthetic genes required for Gb3 synthesis as has been previously shown (25)(26)(27), but also identify novel positive regulatory genes that control membrane SL levels.…”

Section: Genome-wide Crispr/cas9 Screen For Positive Regulators Of Slmentioning

confidence: 99%

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A genome-wide CRISPR/Cas9 screen reveals that the aryl hydrocarbon receptor stimulates sphingolipid levels

Majumder

Kono

Lee

et al. 2020

Journal of Biological Chemistry

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Sphingolipid biosynthesis generates lipids for membranes and signaling that are crucial for many developmental and physiological processes. In some cases, large amounts of specific sphingolipids must be synthesized for specialized physiological functions, such as during axon myelination. How sphingolipid synthesis is regulated to fulfill these physiological requirements is not known. To identify genes that positively regulate membrane sphingolipid levels, here we employed a genome-wide CRISPR/Cas9 loss-of-function screen in HeLa cells using selection for resistance to Shiga toxin, which uses a plasma membrane-associated glycosphingolipid, globotriaosylceramide (Gb3), for its uptake. The screen identified several genes in the sphingolipid biosynthetic pathway that are required for Gb3 synthesis, and it also identified the aryl hydrocarbon receptor (AHR), a ligand-activated transcription factor widely involved in development and physiology, as being required for Gb3 biosynthesis. AHR bound and activated the gene promoter of serine palmitoyltransferase small subunit A (SPTSSA), which encodes a subunit of the serine palmitoyltransferase that catalyzes the first and rate-limiting step in de novo sphingolipid biosynthesis. AHR knockout HeLa cells exhibited significantly reduced levels of cell-surface Gb3, and both AHR knockout HeLa cells and tissues from Ahr knockout mice displayed decreased sphingolipid content as well as significantly reduced expression of several key genes in the sphingolipid biosynthetic pathway. The sciatic nerve of Ahr knockout mice exhibited both reduced ceramide content and reduced myelin thickness. These results indicate that AHR up-regulates sphingolipid levels and is important for full axon myelination, which requires elevated levels of membrane sphingolipids.

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Section: Genome-wide Crispr/cas9 Screen For Positive Regulators Of Slmentioning

confidence: 66%

Section: Genome-wide Crispr/cas9 Screen For Positive Regulators Of Slmentioning

confidence: 99%

A genome-wide CRISPR/Cas9 screen reveals that the aryl hydrocarbon receptor stimulates sphingolipid levels

Majumder

Kono

Lee

et al. 2020

Journal of Biological Chemistry

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“…GS28 and STX5 are components of the Golgi target-membrane-bound (t)-SNARE-complex 40 , and UNC50 is a factor involved in intra-cellular trafficking 41, 42 . These genes were previously found in several CRISPR screens for host factors required for actions of ricin 43 , Shiga toxin 44 , and for regulators of the cell surface localization of galectin-3 45 . Their defects induced mildly positive T5 mAb staining, decreased CTxB staining, and slightly increased levels of staining by GS-II lectin.…”

Section: Resultsmentioning

confidence: 92%

Cross-talks of glycosylphosphatidylinositol biosynthesis with glycosphingolipid biosynthesis and ER-associated degradation

Wang

Maeda

Liu

et al. 2019

Preprint

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16 17 18 Glycosylphosphatidylinositol (GPI)-anchored proteins and glycosphingolipids interact with 19 each other in the mammalian plasma membranes, forming dynamic microdomains. How their 20interaction starts in the cells has been unclear. Here, based on a genome-wide CRISPR-Cas9 21 genetic screen for genes required for GPI side-chain modification by galactose in the Golgi 22 apparatus, we report that b1,3-galactosyltransferase 4 (B3GALT4), also called GM1 23 ganglioside synthase, additionally functions in transferring galactose to the N-24 acetylgalactosamine side-chain of GPI. Furthermore, B3GALT4 requires lactosylceramide 25 for the efficient GPI side-chain galactosylation. Thus, our work demonstrates previously 26 unexpected evolutionary and functional relationships between GPI-anchored proteins and 27 glycosphingolipids in the Golgi. Through the same screening, we also show that GPI 28 biosynthesis in the endoplasmic reticulum (ER) is severely suppressed by ER-associated 29 degradation to prevent GPI accumulation when the transfer of synthesized GPI to proteins is 30 defective. Our data demonstrates cross-talks of GPI biosynthesis with glycosphingolipid 31 biosynthesis and the ER quality control system. 32 33CRISPR genome-wide screen. 36 37 Glycosylphosphatidylinositol (GPI) is a complex glycolipid for post-translational 38 modification of many cell-surface proteins in eukaryotic cells 1 . To date, more than 150 39 human proteins have been confirmed as GPI-anchored proteins (GPI-APs) 2 . The structure of 40 the core backbone of GPI, which is conserved in eukaryotic organisms, is EtNP-6Mana-41 2Mana-6Mana-4GlcNa-6Inositol-phospholipid (where EtNP, Man and GlcN are 42 ethanolamine phosphate, mannose and glucosamine, respectively) ( Fig. 1a). GPI is 43 synthesized in the endoplasmic reticulum (ER) followed by transfer of GPI to proteins that 44 have a C-terminal GPI-attachment signal peptide. The GPI-attachment signal peptide is 45 removed and replaced with GPI by the GPI-transamidase (GPI-Tase) complex to form 46 immature GPI-APs. Nascent GPI-APs undergo structural remodeling in the ER and the Golgi 47 apparatus. The inositol-linked acyl chain is deacylated and the EtNP side branch is removed 48 from the second Man (Man2) for efficient ER to Golgi transport 3-5 . In the Golgi, GPI fatty 49 acid remodeling occurs, in which an sn-2-linked unsaturated fatty acyl chain is removed and 50 reacylated with a saturated chain, usually stearic acid 6,7 . Fatty acid remodeling is crucial for 51 lipid-raft association of GPI, a feature of GPI-APs 8 . 52 53The structural variation of GPI anchors is introduced by side-chain modifications 1 . Structural 54 studies of GPIs from some mammalian GPI-APs indicated that the first mannose (Man1) is 55 often modified with β1,4-linked N-acetylgalactosamine (GalNAc) 9,10 . This modification is 56 mediated by PGAP4 (Post-GPI attachment to proteins 4 also known as TMEM246), a 57 recently identified Golgi-resident, GPI-specific GalNAc-transferase 11 . The GalNAc side-58 chain can be furth...

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“…What is the relevance of multiple phenotypes targeted by pore-forming toxins, namely, how do pore-forming toxins lead to the fission or vacuolation of the ER (Brito, Cabanes, Sarmento Mesquita, & Sousa, 2019;Gonzalez et al, 2018;Mesquita et al, 2017)? Or how further can we exploit toxins to screen for regulators of organelle function and biosynthetic pathways (Tian et al, 2018)? Combined with model organisms, tailored pharmacological treatments, and emerging fine-tuned genetic manipulations, bacterial toxins will continue to reveal clever strategies that help us to dissect and identify fundamental, and exceedingly precise, properties of membrane trafficking.…”

Section: Future Perspectivesmentioning

confidence: 99%

Mammalian membrane trafficking as seen through the lens of bacterial toxins

Mesquita

Goot

Sergeeva

2020

Cellular Microbiology

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A fundamental question of eukaryotic cell biology is how membrane organelles are organised and interact with each other. Cell biologists address these questions by characterising the structural features of membrane compartments and the mechanisms that coordinate their exchange. To do so, they must rely on variety of cargo molecules and treatments that enable targeted perturbation, localisation, and labelling of specific compartments. In this context, bacterial toxins emerged in cell biology as paradigm shifting molecules that enabled scientists to not only study them from the side of bacterial infection but also from the side of the mammalian host. Their selectivity, potency, and versatility made them exquisite tools for uncovering much of our current understanding of membrane trafficking mechanisms. Here, we will follow the steps that lead toxins until their intracellular targets, highlighting how specific events helped us comprehend membrane trafficking and establish the fundamentals of various cellular organelles and processes. Bacterial toxins will continue to guide us in answering crucial questions in cellular biology while also acting as probes for new technologies and applications.

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Genome-wide CRISPR screens for Shiga toxins and ricin reveal Golgi proteins critical for glycosylation

Cited by 72 publications

References 60 publications

A genome-wide CRISPR/Cas9 screen reveals that the aryl hydrocarbon receptor stimulates sphingolipid levels

A genome-wide CRISPR/Cas9 screen reveals that the aryl hydrocarbon receptor stimulates sphingolipid levels

Cross-talks of glycosylphosphatidylinositol biosynthesis with glycosphingolipid biosynthesis and ER-associated degradation

Mammalian membrane trafficking as seen through the lens of bacterial toxins

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