血清淀粉样蛋白 A 和 Janus 激酶 2 在糖尿病肾病小鼠模型中的作用。
Serum amyloid A and Janus kinase 2 in a mouse model of diabetic kidney disease.
机构信息
Providence Medical Research Center, Providence Health Care, Spokane, Washington, United States of America.
Internal Medicine, University of Michigan, Ann Arbor, Michigan, United States of America.
出版信息
PLoS One. 2019 Feb 14;14(2):e0211555. doi: 10.1371/journal.pone.0211555. eCollection 2019.
BACKGROUND
Serum amyloid A (SAA), a potent inflammatory mediator, and Janus kinase 2 (JAK2), an intracellular signaling kinase, are increased by diabetes. The aims were to elucidate: 1) a JAK2-mediated pathway for increased SAA in the kidneys of diabetic mice; 2) a JAK2-SAA pathway for inflammation in podocytes.
METHODS
Akita diabetic mice (129S6) with podocyte JAK2 overexpression and angiotensin II infusion (4 weeks) were given a JAK1,2 inhibitor (LY03103801, 3 mg/kg/day orally for the last two weeks). Kidneys were immunostained for SAA isoform 3 (SAA3). SAA3 knockout and control mouse podocytes were exposed to advanced glycation end products (AGE) or exogenous SAA with JAK2 inhibition (Tyrphostin AG 490, 50μM). JAK2 activity (phosphorylation, Western blot, 1 hour) and mRNA for SAA3 and associated inflammatory genes (Cxcl5, Ccl2, and Ccl5) were measured by RT-PCR (20 hours).
RESULTS
SAA3 protein was present throughout the diabetic kidney, and podocyte JAK2 overexpression increased tubulointerstitial SAA3 compared to wild type diabetic controls, 43% versus 14% (p = 0.007); JAK1,2 inhibition attenuated the increase in SAA3 to 15% (p = 0.003). Urine albumin-to-creatinine ratio (r = 0.49, p = 0.03), mesangial index (r = 0.64, p = 0.001), and glomerulosclerosis score (r = 0.51, p = 0.02) were associated with SAA3 immunostaining scores across mouse groups. Exposing podocytes to AGE or exogenous SAA increased JAK2 activity within one hour and mRNA for associated inflammatory genes after 20 hours. JAK2 inhibition reduced SAA3 mRNA expression in podocytes exposed to AGE or SAA. SAA3 knockout podocytes had >85% lower AGE-induced inflammatory genes.
CONCLUSION
JAK1,2 inhibition reduced SAA and histological features of DKD in podocyte JAK2-overexpressing mice. In podocytes exposed to a diabetes-like condition, JAK2 inhibition reduced expression of SAA, while SAA knockout blocked expression of associated pro-inflammatory mediators. SAA may promote JAK2-dependent inflammation in the diabetic kidney.
背景
血清淀粉样蛋白 A(SAA)是一种有效的炎症介质,Janus 激酶 2(JAK2)是一种细胞内信号激酶,它们在糖尿病患者中增加。目的是阐明:1)糖尿病小鼠肾脏中 JAK2 介导的 SAA 增加途径;2)足细胞中 JAK2-SAA 途径的炎症反应。
方法
阿替卡糖尿病小鼠(129S6)过表达足细胞 JAK2 并输注血管紧张素 II(4 周),然后给予 JAK1、2 抑制剂(LY03103801,每天口服 3 毫克/千克,持续最后两周)。对 SAA 同工型 3(SAA3)进行免疫染色。用晚期糖基化终产物(AGE)或外源性 SAA 暴露 SAA3 敲除和对照小鼠足细胞,并使用 JAK2 抑制剂(Tyrphostin AG 490,50μM)。通过 RT-PCR(20 小时)测量 JAK2 活性(磷酸化,Western blot,1 小时)和 SAA3 及相关炎症基因(Cxcl5、Ccl2 和 Ccl5)的 mRNA。
结果
SAA3 蛋白存在于整个糖尿病肾脏中,与野生型糖尿病对照组相比,足细胞 JAK2 过表达增加了肾小管间质 SAA3,分别为 43%和 14%(p = 0.007);JAK1、2 抑制将 SAA3 的增加降低至 15%(p = 0.003)。尿白蛋白/肌酐比值(r = 0.49,p = 0.03)、系膜指数(r = 0.64,p = 0.001)和肾小球硬化评分(r = 0.51,p = 0.02)与各组小鼠的 SAA3 免疫染色评分相关。将足细胞暴露于 AGE 或外源性 SAA 中会在一小时内增加 JAK2 活性,并在 20 小时后增加相关炎症基因的 mRNA。在暴露于 AGE 或 SAA 的足细胞中,JAK2 抑制降低了 SAA3 mRNA 的表达。SAA3 敲除的足细胞中 AGE 诱导的炎症基因降低了>85%。
结论
JAK1、2 抑制减少了 JAK2 过表达的足细胞糖尿病肾病中的 SAA 和组织学特征。在暴露于糖尿病样条件的足细胞中,JAK2 抑制降低了 SAA 的表达,而 SAA 敲除阻止了相关促炎介质的表达。SAA 可能在糖尿病肾脏中促进 JAK2 依赖性炎症反应。
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