| Literature DB >> 33628203 |
Rongqing Li1,2,3, Na Sun1,2,3, Xin Chen1,2, Xueqin Li1,2, Jie Zhao1,2, Wanpeng Cheng1,2, Hui Hua1,2, Masahiko Fukatsu3, Hirotaka Mori3, Hiroshi Takahashi3, Hiroshi Ohkawara3, Miwa Fukami3, Masatoshi Okamoto4, Yoichi Hamazaki5, Kuiyang Zheng1,2, Jing Yang1,2, Takayuki Ikezoe3.
Abstract
A substitution mutation of valine to phenylalanine at codon encoding position 617 of the Janus kinase 2 (JAK2) gene (JAK2V617F ) has been detected in myeloid cells of some individuals with higher levels of proinflammatory cytokine production such as interleukin (IL)-6. However, the mechanisms by which JAK2V617F mutation mediating those cytokines remain unclear. We, therefore, established JAK2V617F -expressing murine macrophages (JAK2V617F macrophages) and found that the levels of p-STAT3 were markedly elevated in JAK2V617F macrophages in association with an increase in IL-6 production. However, inhibition of STAT3 by C188-9 significantly decreased the production of IL-6. Furthermore, the JAK2V617F mutation endowed macrophages with an elevated glycolytic phenotype in parallel with aberrant expression of PKM1. Interestingly, silencing of PKM1 inactivated STAT3 in parallel with reduced IL-6 production. In contrast, ectopic expression of PKM1 elevated IL-6 production via STAT3 activation. Importantly, the JAK2V617F mutation contributed to PKM1 protein stabilization via blockade of lysosomal-dependent degradation via chaperone-mediated autophagy (CMA), indicating that the JAK2V617F mutation could protect PKM1 from CMA-mediated degradation, leading to activation of STAT3 and promoting IL-6 production.Entities:
Keywords: IL-6; JAK2V617F; PKM1; STAT3; glycolysis
Year: 2021 PMID: 33628203 PMCID: PMC7897702 DOI: 10.3389/fimmu.2020.589048
Source DB: PubMed Journal: Front Immunol ISSN: 1664-3224 Impact factor: 7.561