FFAR1 激活可减轻人呼吸道平滑肌细胞中组胺诱导的肌球蛋白轻链磷酸化和皮质张力发展。
FFAR1 activation attenuates histamine-induced myosin light chain phosphorylation and cortical tension development in human airway smooth muscle cells.
机构信息
The Joint Graduate Program in Toxicology, Department of Pharmacology & Toxicology, Ernest Mario School of Pharmacy, Piscataway, USA.
Rutgers Institute for Translational Medicine & Science, New Brunswick, NJ, 08901, USA.
出版信息
Respir Res. 2020 Nov 30;21(1):317. doi: 10.1186/s12931-020-01584-w.
BACKGROUND
Activation of free fatty acid receptors (FFAR1 and FFAR4) which are G protein-coupled receptors (GPCRs) with established (patho)physiological roles in a variety of obesity-related disorders, induce human airway smooth muscle (HASM) cell proliferation and shortening. We reported amplified agonist-induced cell shortening in HASM cells obtained from obese lung donors. We hypothesized that FFAR1 modulate excitation-contraction (EC) coupling in HASM cells and play a role in obesity-associated airway hyperresponsiveness.
METHODS
In HASM cells pre-treated (30 min) with FFAR1 agonists TAK875 and GW9508, we measured histamine-induced Ca mobilization, myosin light chain (MLC) phosphorylation, and cortical tension development with magnetic twisting cytometry (MTC). Phosphorylation of MLC phosphatase and Akt also were determined in the presence of the FFAR1 agonists or vehicle. In addition, the effects of TAK875 on MLC phosphorylation were measured in HASM cells desensitized to βAR agonists by overnight salmeterol treatment. The inhibitory effect of TAK875 on MLC phosphorylation was compared between HASM cells from age and sex-matched non-obese and obese human lung donors. The mean measurements were compared using One-Way ANOVA with Dunnett's test for multiple group comparisons or Student's t-test two-group comparison. For cortical tension measurements by magnetic twisted cytometry, mixed effect model using SAS V.9.2 was applied. Means were considered significant when p ≤ 0.05.
RESULTS
Unexpectedly, we found that TAK875, a synthetic FFAR1 agonist, attenuated histamine-induced MLC phosphorylation and cortical tension development in HASM cells. These physiological outcomes were unassociated with changes in histamine-evoked Ca flux, protein kinase B (AKT) activation, or MLC phosphatase inhibition. Of note, TAK875-mediated inhibition of MLC phosphorylation was maintained in βAR-desensitized HASM cells and across obese and non-obese donor-derived HASM cells.
CONCLUSIONS
Taken together, our findings identified the FFAR1 agonist TAK875 as a novel bronchoprotective agent that warrants further investigation to treat difficult-to-control asthma and/or airway hyperreactivity in obesity.
背景
游离脂肪酸受体(FFAR1 和 FFAR4)是具有多种肥胖相关疾病中已建立的(病理)生理作用的 G 蛋白偶联受体(GPCR),其激活可诱导人气道平滑肌(HASM)细胞增殖和缩短。我们报道了从肥胖肺供体获得的 HASM 细胞中,激动剂诱导的细胞缩短作用被放大。我们假设 FFAR1 调节 HASM 细胞中的兴奋-收缩(EC)偶联,并在肥胖相关的气道高反应性中发挥作用。
方法
在 HASM 细胞用 FFAR1 激动剂 TAK875 和 GW9508 预处理(30 分钟)后,我们使用磁扭动力学(MTC)测量组胺诱导的 Ca 动员、肌球蛋白轻链(MLC)磷酸化和皮质张力发展。还在 FFAR1 激动剂或载体存在下测定肌球蛋白轻链磷酸酶和 Akt 的磷酸化。此外,通过过夜沙美特罗处理使 HASM 细胞对βAR 激动剂脱敏,测量 TAK875 对 MLC 磷酸化的作用。TAK875 对 MLC 磷酸化的抑制作用在年龄和性别匹配的非肥胖和肥胖人肺供体来源的 HASM 细胞之间进行比较。使用 One-Way ANOVA 进行均值比较,并使用 Dunnett 检验进行多组比较或 Student's t-test 进行两组比较。对于磁扭动力学测量的皮质张力,使用 SAS V.9.2 中的混合效应模型。当 p≤0.05 时,认为均值具有统计学意义。
结果
出乎意料的是,我们发现合成的 FFAR1 激动剂 TAK875 减弱了 HASM 细胞中组胺诱导的 MLC 磷酸化和皮质张力发展。这些生理结果与组胺诱导的 Ca 通量、蛋白激酶 B(AKT)激活或 MLC 磷酸酶抑制的变化无关。值得注意的是,TAK875 介导的 MLC 磷酸化抑制在βAR 脱敏的 HASM 细胞中以及肥胖和非肥胖供体来源的 HASM 细胞中均得到维持。
结论
综上所述,我们的发现确定了 FFAR1 激动剂 TAK875 作为一种新型的支气管保护剂,值得进一步研究,以治疗肥胖相关的难以控制的哮喘和/或气道高反应性。
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