中华劳动卫生职业病杂志
中華勞動衛生職業病雜誌
중화노동위생직업병잡지
CHINESE JOURNAL OF INDUSTRIAL HYGIENE AND OCCUPATIONAL DISEASES
2010年
4期
241-245
,共5页
刘海峰%张凤梅%刘秉慈%贾效伟%叶萌
劉海峰%張鳳梅%劉秉慈%賈效偉%葉萌
류해봉%장봉매%류병자%가효위%협맹
石英%DNA连接酶类%DNA损伤%彗星试验%DNA修复
石英%DNA連接酶類%DNA損傷%彗星試驗%DNA脩複
석영%DNA련접매류%DNA손상%혜성시험%DNA수복
Quartz%DNA ligases%DNA damage%Comet assay%DNA repair
目的 探讨磷脂酰肌醇-3激酶(phosphatidylinositol 3 kinase,PI3K)在石英致人胚肺成纤维细胞(HELF)DNA双链断裂修复中的作用.方法 用200μg/ml的石英刺激HELF和用显性失活突变体抑制P13K功能的HELF(DN-Δp85)不同时间.免疫印迹法检测磷酸化H2AX(γH2AX)的水平以及DNA依赖性蛋白激酶(DNA-dependent protein kinase,DNA-PK)的组成成分Ku70、Ku8和DNA-PKcs的蛋白水平,并用Image-Pro plus 6.0软件对条带光强度进行半定量分析.中性彗星试验检测DNA双链断裂损伤,用彗尾DNA百分含量值观察DNA双链断裂损伤程度变化,并计算DNA修复能力.结果 γH2AX的水平在石英刺激3 h明显增高,12 h达峰值,24 h下降.与HELF相比,石英诱导的DN-Δp85细胞γH2AX水平增高受到抑制.石英刺激HELF和DN-ΔP85细胞12 h组Ku70、Ku80和DNA-PKcs的蛋白水平(0.58±0.09、0.95±0.21、0.55±0.06,0.37±0.14、0.55±0.17、0.52±0.07)均高于相应的无石英刺激组(0.26±0.10、0.69±0.26、0.43±0.11,0.11±0.07、0.27±0.14、0.39±0.07),差异有统计学意义(P<0.05).与石英刺激HELF 12 h组比较,石英刺激DN-ΔP85 12 h组的Ku70、Ku80蛋白水平增高受到抑制,差异均有统计学意义(P<0.05).石英刺激的HELF12 h组和DN-Δp85 12h组的彗尾DNA百分含量分别为9.78±1.15和11.79±4.90,明显高于同细胞系的无石英刺激组(2.40±0.69,3.31±1.35),差异有统计学意义(P<0.05);与石英刺激HELF 12 h组相比,石英刺激HELF细胞24 h组彗尾DNA百分含量明显降低(4.19±0.47),差异有统计学意义(P<0.05).石英刺激DN-Δp85 24 h组的彗尾DNA百分含量为(7.58±4.32),明显高于无石英刺激DN-Δp85组和石英刺激HELF 24 h组,差异有统计学意义(P<0.05).HELF的DNA修复能力为75.74%,DN-Δp85的DNA修复能力为49.64%.结论 石英可诱导DNA双链断裂损伤,PI3K与DNA损伤修复有关,通过调节Ku70和Ku80的水平,可促进石英诱导的DNA双链断裂损伤的修复.
目的 探討燐脂酰肌醇-3激酶(phosphatidylinositol 3 kinase,PI3K)在石英緻人胚肺成纖維細胞(HELF)DNA雙鏈斷裂脩複中的作用.方法 用200μg/ml的石英刺激HELF和用顯性失活突變體抑製P13K功能的HELF(DN-Δp85)不同時間.免疫印跡法檢測燐痠化H2AX(γH2AX)的水平以及DNA依賴性蛋白激酶(DNA-dependent protein kinase,DNA-PK)的組成成分Ku70、Ku8和DNA-PKcs的蛋白水平,併用Image-Pro plus 6.0軟件對條帶光彊度進行半定量分析.中性彗星試驗檢測DNA雙鏈斷裂損傷,用彗尾DNA百分含量值觀察DNA雙鏈斷裂損傷程度變化,併計算DNA脩複能力.結果 γH2AX的水平在石英刺激3 h明顯增高,12 h達峰值,24 h下降.與HELF相比,石英誘導的DN-Δp85細胞γH2AX水平增高受到抑製.石英刺激HELF和DN-ΔP85細胞12 h組Ku70、Ku80和DNA-PKcs的蛋白水平(0.58±0.09、0.95±0.21、0.55±0.06,0.37±0.14、0.55±0.17、0.52±0.07)均高于相應的無石英刺激組(0.26±0.10、0.69±0.26、0.43±0.11,0.11±0.07、0.27±0.14、0.39±0.07),差異有統計學意義(P<0.05).與石英刺激HELF 12 h組比較,石英刺激DN-ΔP85 12 h組的Ku70、Ku80蛋白水平增高受到抑製,差異均有統計學意義(P<0.05).石英刺激的HELF12 h組和DN-Δp85 12h組的彗尾DNA百分含量分彆為9.78±1.15和11.79±4.90,明顯高于同細胞繫的無石英刺激組(2.40±0.69,3.31±1.35),差異有統計學意義(P<0.05);與石英刺激HELF 12 h組相比,石英刺激HELF細胞24 h組彗尾DNA百分含量明顯降低(4.19±0.47),差異有統計學意義(P<0.05).石英刺激DN-Δp85 24 h組的彗尾DNA百分含量為(7.58±4.32),明顯高于無石英刺激DN-Δp85組和石英刺激HELF 24 h組,差異有統計學意義(P<0.05).HELF的DNA脩複能力為75.74%,DN-Δp85的DNA脩複能力為49.64%.結論 石英可誘導DNA雙鏈斷裂損傷,PI3K與DNA損傷脩複有關,通過調節Ku70和Ku80的水平,可促進石英誘導的DNA雙鏈斷裂損傷的脩複.
목적 탐토린지선기순-3격매(phosphatidylinositol 3 kinase,PI3K)재석영치인배폐성섬유세포(HELF)DNA쌍련단렬수복중적작용.방법 용200μg/ml적석영자격HELF화용현성실활돌변체억제P13K공능적HELF(DN-Δp85)불동시간.면역인적법검측린산화H2AX(γH2AX)적수평이급DNA의뢰성단백격매(DNA-dependent protein kinase,DNA-PK)적조성성분Ku70、Ku8화DNA-PKcs적단백수평,병용Image-Pro plus 6.0연건대조대광강도진행반정량분석.중성혜성시험검측DNA쌍련단렬손상,용혜미DNA백분함량치관찰DNA쌍련단렬손상정도변화,병계산DNA수복능력.결과 γH2AX적수평재석영자격3 h명현증고,12 h체봉치,24 h하강.여HELF상비,석영유도적DN-Δp85세포γH2AX수평증고수도억제.석영자격HELF화DN-ΔP85세포12 h조Ku70、Ku80화DNA-PKcs적단백수평(0.58±0.09、0.95±0.21、0.55±0.06,0.37±0.14、0.55±0.17、0.52±0.07)균고우상응적무석영자격조(0.26±0.10、0.69±0.26、0.43±0.11,0.11±0.07、0.27±0.14、0.39±0.07),차이유통계학의의(P<0.05).여석영자격HELF 12 h조비교,석영자격DN-ΔP85 12 h조적Ku70、Ku80단백수평증고수도억제,차이균유통계학의의(P<0.05).석영자격적HELF12 h조화DN-Δp85 12h조적혜미DNA백분함량분별위9.78±1.15화11.79±4.90,명현고우동세포계적무석영자격조(2.40±0.69,3.31±1.35),차이유통계학의의(P<0.05);여석영자격HELF 12 h조상비,석영자격HELF세포24 h조혜미DNA백분함량명현강저(4.19±0.47),차이유통계학의의(P<0.05).석영자격DN-Δp85 24 h조적혜미DNA백분함량위(7.58±4.32),명현고우무석영자격DN-Δp85조화석영자격HELF 24 h조,차이유통계학의의(P<0.05).HELF적DNA수복능력위75.74%,DN-Δp85적DNA수복능력위49.64%.결론 석영가유도DNA쌍련단렬손상,PI3K여DNA손상수복유관,통과조절Ku70화Ku80적수평,가촉진석영유도적DNA쌍련단렬손상적수복.
Objective To study the role of Phosphatidylinositol 3 kinase(PI3K)in silica-induced DNA double strand break repair in human embryo lung fibroblasts(HELF).Methods Control HELF cells and DN-Δp85(HELF transfected with Dominant negative mutant of PI3K)were treated with 200μg/ml, silica for different times.The expression levels of phosphor-H2AX(H2AX),Ku70,Ku80 and DNA-PKcs were de-termined by Western blot.Furthermore,DNA double strand breaks were measuled by neutral comet assay after cells were treated with 200 μg/ml silica for 0,12 and 24 h.Results After treatment with 200 μg/ml silica for different times,the levels of H2AX were increased in a time-dependent manner and the expression levels of H2AX were obviously suppressed in DN-Δp85 compared with control cells.The levels of Ku70 and Ku80were also significantly suppressed in DN-Δp85(0.37±20.14,0.55±0.17)compared with control cells(0.58±0.09,0.95±0.21)after treatment with 200 μg/ml silica for 12 h(P<0.05).Both the percentage of tail DNA in HELF and DN-Δp85 increased significantly at 12 h(9.78±1.15,11.79±4.90)compared with groups without treatment with silica(2.40±0.69,3.31±1.35)and then decreased at 24 h(4.19±0.47,7.58±4.32),but only the decrease of HELF at 24 h was significant compared with HELF at 12 h(P<0.05).DNA repair competence of HELF was 75.74%and that of DN-Δp85 declined to 49.64%.Conclusion Silica dust can induce DNA double strand breaks in human embryo lung fibroblasts.P13K might play a role in silica-induced DNA double strand break repair by regulating the expression levels of Ku70 and Ku80.