Publications by authors named "Y M Chook"
Core histones, synthesized and processed in the cytoplasm, must be chaperoned as they are transported into the nucleus for nucleosome assembly. The importin Kap114 transports H2A-H2B into the yeast nucleus, where RanGTP facilitates histone release. Kap114 and H2A-H2B also bind the histone chaperone Nap1, but how Nap1 and Kap114 cooperate in transport and nucleosome assembly remains unclear.
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- The nuclear export receptor XPO1 is commonly overexpressed in cancer cells, leading to mislocalization of important proteins; the inhibitor selinexor reverses this effect by blocking XPO1-cargo binding.
- Selinexor triggers the degradation of XPO1 through a specific mechanism involving the cullin-RING E3 ubiquitin ligase (CRL) system and its substrate receptor ASB8.
- Research using cryogenic electron microscopy revealed that selinexor stabilizes XPO1 in a unique conformation, allowing ASB8 to bind effectively and facilitate ubiquitination, showcasing a new method of protein degradation that differs from previously known molecular glue strategies.
Gene expression in response to environmental stimuli is dependent on nuclear localization of key signaling components, which can be tightly regulated by phosphorylation. This is exemplified by the phosphate-sensing transcription factor Pho4, which requires phosphorylation for nuclear export by the yeast exportin Msn5. Unlike the traditional hydrophobic nuclear export signal (NES) utilized by the Exportin-1/XPO1 system, cryogenic-electron microscopy structures reveal that Pho4 presents a novel, phosphorylated 35-residue NES that interacts with the concave surface of Msn5 through two Pho4 phospho-serines that align with two Msn5 basic patches, unveiling a previously unknown mechanism of phosphate-specific recognition.
View Article and Find Full Text PDFIn this issue, the discovery by Yang et al. (https://doi.org/10.
View Article and Find Full Text PDFDisease-causing missense mutations that occur within structurally and functionally unannotated protein regions can guide researchers to new mechanisms of protein regulation and dysfunction. Here, we report that the thrombocytopenia-, myelodysplastic syndromes-, and leukemia-associated P214L mutation in the transcriptional regulator ETV6 creates an XPO1-dependent nuclear export signal to cause protein mislocalization. Strategies to disrupt XPO1 activity fully restore ETV6 P214L protein nuclear localization and transcription regulation activity.
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