国际肿瘤学杂志
國際腫瘤學雜誌
국제종류학잡지
JOURNAL OF INTERNATIONAL ONCOLOGY
2009年
12期
946-948
,共3页
张恒兰%温培娥%任霞%孙晓柏%苏恩裕%姜国胜
張恆蘭%溫培娥%任霞%孫曉柏%囌恩裕%薑國勝
장항란%온배아%임하%손효백%소은유%강국성
真菌%多糖类%HL-60细胞%凋亡
真菌%多糖類%HL-60細胞%凋亡
진균%다당류%HL-60세포%조망
Fungi%Polysaccharides%HL-60 cells%Apoptosis
目的 研究真菌Polyporus sp.M05多糖APS-1(一种多孔菌多糖SP.M05-1)和APS-2对白血病细胞HL-60增殖抑制及诱导凋亡作用,并探讨其分子机制.方法 运用活细胞计数法检测多糖的增殖抑制作用并选择药物浓度;碘化啶(PI)染色后利用流式细胞术检测细胞凋亡作用;逆转录聚合酶链反应(RT-PCR)检测凋亡相关基因表达.结果 多糖对HL-60细胞有增殖抑制作用,并随着浓度的增大和作用时间延长作用增强;APS-1作用48 h后凋亡率达47.9%,APS-2作用细胞48 h后凋亡率为26.8%,与阴性对照相比差异有统计学意义(P<0.01);RT-PCR检测到APS-1作用后细胞中Bax、Fas及半胱天冬酶(Caspase)-3基因上调,APS-2作用后细胞中Bax和Caspase-3基因上调,而Fas基因表达无变化.结论 Polyporus sp.M05中提取的多糖APS-1和APS-2对自血病细胞HL-60具有增殖抑制和诱导凋亡作用,APS-1可同时通过线粒体途径和死亡受体途径诱导HL-60细胞凋亡,而APS-2通过线粒体途径诱导HL-60细胞凋亡.
目的 研究真菌Polyporus sp.M05多糖APS-1(一種多孔菌多糖SP.M05-1)和APS-2對白血病細胞HL-60增殖抑製及誘導凋亡作用,併探討其分子機製.方法 運用活細胞計數法檢測多糖的增殖抑製作用併選擇藥物濃度;碘化啶(PI)染色後利用流式細胞術檢測細胞凋亡作用;逆轉錄聚閤酶鏈反應(RT-PCR)檢測凋亡相關基因錶達.結果 多糖對HL-60細胞有增殖抑製作用,併隨著濃度的增大和作用時間延長作用增彊;APS-1作用48 h後凋亡率達47.9%,APS-2作用細胞48 h後凋亡率為26.8%,與陰性對照相比差異有統計學意義(P<0.01);RT-PCR檢測到APS-1作用後細胞中Bax、Fas及半胱天鼕酶(Caspase)-3基因上調,APS-2作用後細胞中Bax和Caspase-3基因上調,而Fas基因錶達無變化.結論 Polyporus sp.M05中提取的多糖APS-1和APS-2對自血病細胞HL-60具有增殖抑製和誘導凋亡作用,APS-1可同時通過線粒體途徑和死亡受體途徑誘導HL-60細胞凋亡,而APS-2通過線粒體途徑誘導HL-60細胞凋亡.
목적 연구진균Polyporus sp.M05다당APS-1(일충다공균다당SP.M05-1)화APS-2대백혈병세포HL-60증식억제급유도조망작용,병탐토기분자궤제.방법 운용활세포계수법검측다당적증식억제작용병선택약물농도;전화정(PI)염색후이용류식세포술검측세포조망작용;역전록취합매련반응(RT-PCR)검측조망상관기인표체.결과 다당대HL-60세포유증식억제작용,병수착농도적증대화작용시간연장작용증강;APS-1작용48 h후조망솔체47.9%,APS-2작용세포48 h후조망솔위26.8%,여음성대조상비차이유통계학의의(P<0.01);RT-PCR검측도APS-1작용후세포중Bax、Fas급반광천동매(Caspase)-3기인상조,APS-2작용후세포중Bax화Caspase-3기인상조,이Fas기인표체무변화.결론 Polyporus sp.M05중제취적다당APS-1화APS-2대자혈병세포HL-60구유증식억제화유도조망작용,APS-1가동시통과선립체도경화사망수체도경유도HL-60세포조망,이APS-2통과선립체도경유도HL-60세포조망.
Objective To detect the proliferation inhibition and apoptosis of HL-60 cell induced by APS-1 and APS-2 isolated from Polyporus sp. M05 and to investigate its mechanism. Methods The proliferation inhibition was detected by living cells count method,and chosed proper concentration.Flow cytometry with propidium iodide staining was used to detect cell apoptosis. Semi-quantitative RT-PCR was used to detect the expression of apoptosis related gene. Results APS-1 and APS-2 could significantly inhibit the proliferation of HL-60 cells on a time and dose dependent manner. Apoptosis ratio increased to 47. 9% and 26. 8% after HL-60 cells were exposed to APS-1 and APS-2 respectively for 48 h,and the differences had statistical significance (P <0.01). After being induced by APS-1,mRNA of Bax,Fas,Caspase-3 was upregulated. And after being induced by APS-2,mRNA of Bax,Caspase-3 was upregulated,while Fas mRNA did not change. Conclusion APS-1 and APS-2 can inhibit the proliferation and induce apoptosis of HL-60 cells. Mechanism of HL-60 cell apoptosis induced by APS-1 is related to both mitochondrial pathway and Fas signaling pathway,while apoptosis induced by APS-2 is only related to mitochondrial pathway.
