Alterations of monocyte NF-κB p65/RelA signaling in a cohort of older medical patients, age-matched controls, and healthy young adults

Juliette Tavenier; Line Jee Hartmann Rasmussen; Morten Baltzer Houlind; Aino Leegaard Andersen; Inge Panum; Ove Andersen; Janne Petersen; Anne Langkilde; Jan O. Nehlin

摘要

Altered monocyte NF-κB signaling is a possible cause of inflammaging and driver of aging, however, evidence from human aging studies is sparse. We assessed monocyte NF-κB signaling across different aging trajectories by comparing healthy older adults to older adults with a recent emergency department (ED) admission and to young adults. We used data from: 52 older (≥65?years) Patients collected upon ED admission and at follow-up 30-days after discharge; 52 age- and sex-matched Older Controls without recent hospitalization; and 60 healthy Young Controls (20–35?years). Using flow cytometry, we assessed basal NF-κB phosphorylation (pNF-κB p65/RelA; Ser529) and induction of pNF-κB following stimulation with LPS or TNF-α in monocytes. We assessed frailty (FI-OutRef), physical and cognitive function, and plasma levels of IL-6, IL-18, TNF-α, and soluble urokinase plasminogen activator receptor. Patients at follow-up were frailer, had higher levels of inflammatory markers and decreased physical and cognitive function than Older Controls. Patients at follow-up had higher basal pNF-κB levels than Older Controls (median fluorescence intensity (MFI): 125, IQR: 105–153 vs. MFI: 80, IQR: 71–90, p??0.0001), and reduced pNF-κB induction in response to LPS (mean pNF-κB MFI fold change calculated as the log10 ratio of LPS-stimulation to the PBS-control: 0.10, 95% CI: 0.08 to 0.12 vs. 0.13, 95% CI: 0.10 to 0.15, p?=?0.05) and TNF-α stimulation (0.02, 95% CI: ??0.00 to 0.05 vs. 0.10, 95% CI: 0.08 to 0.12, p??0.0001). Older Controls had higher levels of inflammatory markers than Young Controls, but basal pNF-κB MFI did not differ between Older and Young Controls (MFI: 81, IQR: 70–86; p?=?0.72). Older Controls had reduced pNF-κB induction in response to LPS and TNF-α compared to Young Controls (LPS: 0.40, 95% CI: 0.35 to 0.44, p??0.0001; and TNF-α: 0.33, 95% CI: 0.27 to 0.40, p??0.0001). In Older Controls, basal pNF-κB MFI was associated with FI-OutRef (p?=?0.02). Increased basal pNF-κB activity in monocytes could be involved in the processes of frailty and accelerated aging. Furthermore, we show that monocyte NF-κB activation upon stimulation was impaired in frail older adults, which could result in reduced immune responses and vaccine effectiveness.

机译：改变的单核细胞NF-κB信号传导是可能的炎性和衰老驾驶员的原因，但是来自人类老化研究的证据是稀疏的。通过将健康的老年人与最近的急诊部门（ED）入学和年轻人进行比较，我们通过将健康的老年人与年轻成年人进行比较来评估不同老化轨迹的单核细胞NF-κB信号传导。我们使用的数据来自：52岁（≥65岁）收集的患者在入院时收集和放电后30天的随访; 52年龄和性别匹配的老年人，没有最近的住院治疗;和60名健康的年轻控件（20-35？年）。使用流式细胞术，我们评估了基础NF-κB磷酸化（PNF-κBP65/ RELA; SER529），并在单核细胞中用LPS或TNF-α刺激后诱导PNF-κB。我们评估了IL-6，IL-18，TNF-α和可溶性尿激酶纤溶酶原激活剂受体的脆弱（Fi-Otref），物理和认知功能，以及血浆水平。随访的患者是脆弱的，具有较高水平的炎症标志物，而且具有比老年人的对照减少的身体和认知功能。随访的患者具有比较旧的对照（中位荧光强度（MFI）：125，IQR：105-153与MFI：80，IQR：71-90，P？<0.0001）和响应于LPS（平均PNF-κBMFI折叠变化为LPS-CONVER的LOG10比率，降低PNF-κB诱导：0.10,95％CI：0.08至0.12 Vs.0.13，95％CI：0.10至0.15，p？= 0.05）和TNF-α刺激（0.02,95％CI：0.00至0.05与0.10,95％CI：0.08至0.12，P？<0.0001）。较旧的对照水平较高的炎症标志物比年轻对照较高，但基础PNF-κBMFI在较旧的和年轻控制之间没有差异（MFI：81，IQR：70-86; P？= 0.72）。与幼小对照相比，较旧的对照减少了pNF-κB诱导（LPS：0.40,95％CI：0.35至0.44，p≤0.301;和TNF-α：0.33,95％CI： 0.27至0.40，p？<？0.0001）。在较旧的对照中，基础PNF-κBMFI与FI-OUTREF相关（P？= 0.02）。单核细胞中的基础PNF-κB活性增加可参与脆弱和加速衰老的过程。此外，我们表明，在Frail老年人中，刺激的单核细胞NF-κB活化受损，这可能导致免疫应答和疫苗效果降低。

Alterations of monocyte NF-κB p65/RelA signaling in a cohort of older medical patients, age-matched controls, and healthy young adults

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