华西口腔医学杂志
華西口腔醫學雜誌
화서구강의학잡지
WEST CHINA JOURNAL OF STOMATOLOGY
2013年
6期
565-568
,共4页
魏美荣%李国菊%张达%颜世果%戚向敏
魏美榮%李國菊%張達%顏世果%慼嚮敏
위미영%리국국%장체%안세과%척향민
角质细胞生长因子%细胞凋亡%口腔黏膜上皮细胞
角質細胞生長因子%細胞凋亡%口腔黏膜上皮細胞
각질세포생장인자%세포조망%구강점막상피세포
keratinocyte growth factor%apoptosis%oral mucosal epithelial cells
目的:研究不同浓度角质细胞生长因子(KGF)对口腔黏膜上皮细胞凋亡的作用,为探讨KGF在口腔黏膜病发生发展中的作用提供依据。方法将不同浓度的KGF(对照组0 ng·mL-1,实验1组5 ng·mL-1,实验2组25 ng·mL-1,实验3组50 ng·mL-1)分别加入体外培养的口腔黏膜上皮细胞,培养12、24、48 h后,倒置显微镜下观察其对细胞形态的影响,并用流式细胞仪检测细胞凋亡情况,荧光实时定量检测细胞凋亡相关基因Bcl-2、Bax mRNA的表达水平。结果1)实验组较对照组细胞贴壁明显,且48 h时实验3组细胞核仁明显。2)培养48 h时,4组之间的细胞凋亡率、Bcl-2 mRNA、Bax mRNA表达均有统计学差异,随着KGF浓度的增加,细胞凋亡率和Bax mRNA表达逐渐降低,Bcl-2 mRNA表达逐渐升高(P<0.05)。结论 KGF可通过上调Bcl-2 mRNA和下调Bax mRNA的表达抑制上皮细胞的凋亡。
目的:研究不同濃度角質細胞生長因子(KGF)對口腔黏膜上皮細胞凋亡的作用,為探討KGF在口腔黏膜病髮生髮展中的作用提供依據。方法將不同濃度的KGF(對照組0 ng·mL-1,實驗1組5 ng·mL-1,實驗2組25 ng·mL-1,實驗3組50 ng·mL-1)分彆加入體外培養的口腔黏膜上皮細胞,培養12、24、48 h後,倒置顯微鏡下觀察其對細胞形態的影響,併用流式細胞儀檢測細胞凋亡情況,熒光實時定量檢測細胞凋亡相關基因Bcl-2、Bax mRNA的錶達水平。結果1)實驗組較對照組細胞貼壁明顯,且48 h時實驗3組細胞覈仁明顯。2)培養48 h時,4組之間的細胞凋亡率、Bcl-2 mRNA、Bax mRNA錶達均有統計學差異,隨著KGF濃度的增加,細胞凋亡率和Bax mRNA錶達逐漸降低,Bcl-2 mRNA錶達逐漸升高(P<0.05)。結論 KGF可通過上調Bcl-2 mRNA和下調Bax mRNA的錶達抑製上皮細胞的凋亡。
목적:연구불동농도각질세포생장인자(KGF)대구강점막상피세포조망적작용,위탐토KGF재구강점막병발생발전중적작용제공의거。방법장불동농도적KGF(대조조0 ng·mL-1,실험1조5 ng·mL-1,실험2조25 ng·mL-1,실험3조50 ng·mL-1)분별가입체외배양적구강점막상피세포,배양12、24、48 h후,도치현미경하관찰기대세포형태적영향,병용류식세포의검측세포조망정황,형광실시정량검측세포조망상관기인Bcl-2、Bax mRNA적표체수평。결과1)실험조교대조조세포첩벽명현,차48 h시실험3조세포핵인명현。2)배양48 h시,4조지간적세포조망솔、Bcl-2 mRNA、Bax mRNA표체균유통계학차이,수착KGF농도적증가,세포조망솔화Bax mRNA표체축점강저,Bcl-2 mRNA표체축점승고(P<0.05)。결론 KGF가통과상조Bcl-2 mRNA화하조Bax mRNA적표체억제상피세포적조망。
Objective To study the function of keratinocyte growth factor (KGF) on apoptosis of oral mucosal epithelial cells and to provide a basis for further investigation of the role of KGF in the occurrence and development of oral mucosal diseases. Methods Different concentrations of KGF (control group, 0 ng·mL-1; experiment 1 group, 5 ng·mL-1; experimental 2 group, 25 ng·mL-1; experiment 3 group, 50 ng·mL-1) were added in oral mucosa epithelial cells cultured in vitro. After training for 12, 24, and 48 h, cell morphology was observed under an inverted microscope. Apoptosis was detected by using a flow cytometry instrument, and mRNA expression of apoptosis-related genes Bcl-2 and Bax was detected by using Real-Time fluorescent quantitative detection. Results Cell adherence of the experimental group was more obvious than that of the control group, and the cell nucleolus of the experiment 3 group was obviously cultured at 48 h. After culturing for 48 h, the apoptosis rate and Bcl-2 and Bax mRNA expression among the four groups were statistically significant. The increase of KGF concentration, apoptosis rate, and Bax mRNA expression gradually reduced, whereas Bcl-2 mRNA expression increased (P<0.05). Conclusion KGF may inhibit epithelial cell apoptosis through upregulation of Bcl-2 mRNA and downregulation of Bax mRNA.
