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Salmonellaexploits HLA-B27 and host unfolded protein responses to promote intracellular replication

未折叠蛋白反应 肠沙门氏菌 细胞生物学 人类白细胞抗原 生物 沙门氏菌 抗原 免疫学 内质网 遗传学 细菌
作者
Antony N. Antoniou,Izabela Lenart,Janos Kriston‐Vizi,Takao Iwawaki,Mark Turmaine,Kirsty McHugh,Sadfer Ali,Neil Blake,Paul Bowness,Mona Bajaj‐Elliott,Keith G. Gould,Darren Nesbeth,Simon J. Powis
出处
期刊:Annals of the Rheumatic Diseases [BMJ]
卷期号:78 (1): 74-82 被引量:47
标识
DOI:10.1136/annrheumdis-2018-213532
摘要

Objective Salmonella enterica infections can lead to Reactive Arthritis (ReA), which can exhibit an association with human leucocyte antigen (HLA)-B*27:05, a molecule prone to misfolding and initiation of the unfolded protein response (UPR). This study examined how HLA-B*27:05 expression and the UPR affect the Salmonella life-cycle within epithelial cells. Methods Isogenic epithelial cell lines expressing two copies of either HLA-B*27:05 and a control HLA-B*35:01 heavy chain (HC) were generated to determine the effect on the Salmonella infection life-cycle. A cell line expressing HLA-B*27:05.HC physically linked to the light chain beta-2-microglobulin and a specific peptide (referred to as a single chain trimer, SCT) was also generated to determine the effects of HLA-B27 folding status on S. enterica life-cycle. XBP-1 venus and AMP dependent Transcription Factor (ATF6)-FLAG reporters were used to monitor UPR activation in infected cells. Triacin C was used to inhibit de novo lipid synthesis during UPR, and confocal imaging of ER tracker stained membrane allowed quantification of glibenclamide-associated membrane. Results S. enterica demonstrated enhanced replication with an altered cellular localisation in the presence of HLA-B*27:05.HC but not in the presence of HLA-B*27:05.SCT or HLA-B*35:01. HLA-B*27:05.HC altered the threshold for UPR induction. Salmonella activated the UPR and required XBP-1 for replication, which was associated with endoreticular membrane expansion and lipid metabolism. Conclusions HLA-B27 misfolding and a UPR cellular environment are associated with enhanced Salmonella replication, while Salmonella itself can activate XBP-1 and ATF6. These data provide a potential mechanism linking the life-cycle of Salmonella with the physicochemical properties of HLA-B27 and cellular events that may contribute to ReA pathogenesis. Our observations suggest that the UPR pathway maybe targeted for future therapeutic intervention.
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