中华耳鼻咽喉头颈外科杂志
中華耳鼻嚥喉頭頸外科雜誌
중화이비인후두경외과잡지
Chinese Journal of Otorhinolaryngology Head and Neck Surgery
2015年
10期
829-835
,共7页
王振霖%吕海丽%张名霞%刘俊其%张云云%韩新玲%张秋航
王振霖%呂海麗%張名霞%劉俊其%張雲雲%韓新玲%張鞦航
왕진림%려해려%장명하%류준기%장운운%한신령%장추항
鼻息肉%鼻黏膜%上皮细胞%丝裂原激活蛋白酶类%受体,糖皮质激素%信号传导
鼻息肉%鼻黏膜%上皮細胞%絲裂原激活蛋白酶類%受體,糖皮質激素%信號傳導
비식육%비점막%상피세포%사렬원격활단백매류%수체,당피질격소%신호전도
Nasal polyps%Nasal mucosa%Epithelial cells%Mitogen-activated protein kinase%Receptors,glucocorticoid%Signal transduction
目的 通过体外研究初步探讨鼻息肉黏膜中糖皮质激素受体(glucocortieoid receptor,GR)亚型GRα/GRβ比例降低的上游信号转导机制.方法 以细菌脂多糖(lipopolysaccharide,LPS)体外诱导人鼻息肉黏膜上皮细胞(human nasal epithelia,HNE)构建糖皮质激素抵抗的细胞模型.以Western Blot及荧光定量反转录聚合酶链反应技术检测梯度浓度的LPS诱导前后及MAPK家族信号通路特异性阻断剂干预前后GRα、GRβ和p38MAPK、ERK、JNK信号通路关键酶在蛋白质及核酸水平的表达变化.以SPSS 16.0软件对诱导和干预前后的表达情况采用单因素方差分析.结果 LPS呈浓度和时间依赖性诱导HNE中GRα/GRβ降低,成功建立GRα/GRβ降低的细胞模型.相同浓度梯度的LPS可呈相同规律地诱导HNE中p38MAPK、ERK、JNK信号通路激活.5、10、15 mg/L LPS诱导的p38MAPK、ERK和JNK在mRNA水平的相对表达量(17.14±1.50、22.34±2.78、30.12±1.07,2.51 ±0.13、3.79±0.67、4.41±0.83,25.62±1.77、31.33±1.97、37.25±2.46)均明显高于对照组(7.39±0.31、2.04±0.34、2.38±0.35),差异有统计学意义(x2值分别为15.347、18.331、14.671,P值均<0.01).p38MAPK通路的特异性阻断剂SB203580和JNK通路的特异性阻断剂SP600125均可明显抑制各自信号通路,且同时出现GRα/GRβ增高,SB203580干预后,GRα/GRβ增加更为明显.ERK通路特异性阻断剂PD98059十预后,GRα/GRβ未发现变化.结论 LPS可能通过激活p38MAPK和JNK信号通路诱导体外培养的HNE中GRα/GRβ降低,其中p38MAPK通路较为主要,针对上述信号通路的调节可能有助于改善糖皮质激素抵抗性鼻息肉的治疗效果.
目的 通過體外研究初步探討鼻息肉黏膜中糖皮質激素受體(glucocortieoid receptor,GR)亞型GRα/GRβ比例降低的上遊信號轉導機製.方法 以細菌脂多糖(lipopolysaccharide,LPS)體外誘導人鼻息肉黏膜上皮細胞(human nasal epithelia,HNE)構建糖皮質激素牴抗的細胞模型.以Western Blot及熒光定量反轉錄聚閤酶鏈反應技術檢測梯度濃度的LPS誘導前後及MAPK傢族信號通路特異性阻斷劑榦預前後GRα、GRβ和p38MAPK、ERK、JNK信號通路關鍵酶在蛋白質及覈痠水平的錶達變化.以SPSS 16.0軟件對誘導和榦預前後的錶達情況採用單因素方差分析.結果 LPS呈濃度和時間依賴性誘導HNE中GRα/GRβ降低,成功建立GRα/GRβ降低的細胞模型.相同濃度梯度的LPS可呈相同規律地誘導HNE中p38MAPK、ERK、JNK信號通路激活.5、10、15 mg/L LPS誘導的p38MAPK、ERK和JNK在mRNA水平的相對錶達量(17.14±1.50、22.34±2.78、30.12±1.07,2.51 ±0.13、3.79±0.67、4.41±0.83,25.62±1.77、31.33±1.97、37.25±2.46)均明顯高于對照組(7.39±0.31、2.04±0.34、2.38±0.35),差異有統計學意義(x2值分彆為15.347、18.331、14.671,P值均<0.01).p38MAPK通路的特異性阻斷劑SB203580和JNK通路的特異性阻斷劑SP600125均可明顯抑製各自信號通路,且同時齣現GRα/GRβ增高,SB203580榦預後,GRα/GRβ增加更為明顯.ERK通路特異性阻斷劑PD98059十預後,GRα/GRβ未髮現變化.結論 LPS可能通過激活p38MAPK和JNK信號通路誘導體外培養的HNE中GRα/GRβ降低,其中p38MAPK通路較為主要,針對上述信號通路的調節可能有助于改善糖皮質激素牴抗性鼻息肉的治療效果.
목적 통과체외연구초보탐토비식육점막중당피질격소수체(glucocortieoid receptor,GR)아형GRα/GRβ비례강저적상유신호전도궤제.방법 이세균지다당(lipopolysaccharide,LPS)체외유도인비식육점막상피세포(human nasal epithelia,HNE)구건당피질격소저항적세포모형.이Western Blot급형광정량반전록취합매련반응기술검측제도농도적LPS유도전후급MAPK가족신호통로특이성조단제간예전후GRα、GRβ화p38MAPK、ERK、JNK신호통로관건매재단백질급핵산수평적표체변화.이SPSS 16.0연건대유도화간예전후적표체정황채용단인소방차분석.결과 LPS정농도화시간의뢰성유도HNE중GRα/GRβ강저,성공건립GRα/GRβ강저적세포모형.상동농도제도적LPS가정상동규률지유도HNE중p38MAPK、ERK、JNK신호통로격활.5、10、15 mg/L LPS유도적p38MAPK、ERK화JNK재mRNA수평적상대표체량(17.14±1.50、22.34±2.78、30.12±1.07,2.51 ±0.13、3.79±0.67、4.41±0.83,25.62±1.77、31.33±1.97、37.25±2.46)균명현고우대조조(7.39±0.31、2.04±0.34、2.38±0.35),차이유통계학의의(x2치분별위15.347、18.331、14.671,P치균<0.01).p38MAPK통로적특이성조단제SB203580화JNK통로적특이성조단제SP600125균가명현억제각자신호통로,차동시출현GRα/GRβ증고,SB203580간예후,GRα/GRβ증가경위명현.ERK통로특이성조단제PD98059십예후,GRα/GRβ미발현변화.결론 LPS가능통과격활p38MAPK화JNK신호통로유도체외배양적HNE중GRα/GRβ강저,기중p38MAPK통로교위주요,침대상술신호통로적조절가능유조우개선당피질격소저항성비식육적치료효과.
Objective To explore the upstream signal transduction mechanism responsible for the decrease of the ratio of the two glucocorticoid receptor (GR) subunits (GRα and GRβ) in nasal polyp in vitro.Methods The GRα/GRβ decrease cell model was established by lipopolysaccharide (LPS)-induced human nasal epithelia (HNE) of nasal polyp in vitro.Changes in the protein and mRNA expression of GRα,GRβ and the key enzymes in the p38MAPK, ERK and JNK signal pathways were measured, respectively,before and after being induced with different doses of LPS and specific inhibitors of p38MAPK, JNK and ERK.SPSS 16.0 software (Analysis of variance, ANOVA) was used to analyze the data.Results With the LPS induction, the GRα/GRβ ratio declined in both a time-dependent manner and a concentrationdependent manner in HNE, which demonstrated the successful establishment of a GRα/GRβ decrease model in vitro.After cultured HNE were induced with the same set of LPS, the p38MAPK, ERK and JNK signal pathways were also activated.The mRNA expression of p38MAPK and JNK in each LPS-induced group (17.14±1.50, 22.34±2.78, 30.12 ± 1.07;2.51 ±0.13, 3.79 ±0.67, 4.41 ±0.83;25.62 ± 1.77,31.33 ± 1.97, 37.25 ±2.46)was significantly higher than that(7.39 ±0.31,2.04 ±0.34, 2.38 ±0.35)in the control group (x2 value was 15.347, 18.331, 14.671, all P <0.01).Either a specific inhibitor (SB203580) of the p38MAPK pathway or a specific inhibitor (SP600125) of the JNK pathway increased the GRα/GRβ ratio at the meantime of inhibiting their pathways.SB203580 exhibited a much stronger increase effect on GRα/GRβ ratio than SP600125.The specific inhibitors (PD98059) of ERK had no influence on the expression of GR isoforms.Conclusions The above results demonstrated that the decrease of GRα/GRβ ratio in HNE induced by LPS in vitro is mediated through the p38MAPK and JNK signal pathways.It is possible to improve the treatment effect of GC resistance in nasal polyp by targeting these specific signal pathways.
