中国现代医药杂志
中國現代醫藥雜誌
중국현대의약잡지
MODERN MEDICINE JOURNAL OF CHINA
2014年
6期
1-4
,共4页
邬丽红%陈一强%孔晋亮%黄宏%张瑾钰%蔡双启
鄔麗紅%陳一彊%孔晉亮%黃宏%張瑾鈺%蔡雙啟
오려홍%진일강%공진량%황굉%장근옥%채쌍계
烟曲霉菌%生物膜%金银花%绿原酸
煙麯黴菌%生物膜%金銀花%綠原痠
연곡매균%생물막%금은화%록원산
Aspergillus fumigatus%Biofilm%Honeysuckle%Chlorogenic acid
探讨金银花主要活性成分绿原酸(CRA)对烟曲霉(A.f)生物膜(BF)的体外影响。方法扫描电镜(SEM)鉴定体外烟曲霉BF;二倍稀释法测定绿原酸的最低抑菌浓度(MIC)及最低杀真菌浓度(MFC);各浓度的CRA分别作用于BF 48h后, XTT减低法测定生物膜内菌细胞的代谢活力;结晶紫(CV)法定量生物膜。结果受试菌株经过培养24h、48h后可形成稳定的BF。药物作用48h后,各浓度CRA对菌体代谢活力与空白组相比差异均无统计学意义(P>0.05);较高浓度的CRA组(256、512、1024μg/ml)生物膜量与空白组相比,差异有统计学意义(P<0.05)。结论烟曲霉体外经培养24h、48h后可形成稳定生物膜;金银花主要活性成分绿原酸不能杀死烟曲霉生物膜细胞,但可以抑制生物膜胞外基质的形成,其抑制作用呈浓度依赖性。
探討金銀花主要活性成分綠原痠(CRA)對煙麯黴(A.f)生物膜(BF)的體外影響。方法掃描電鏡(SEM)鑒定體外煙麯黴BF;二倍稀釋法測定綠原痠的最低抑菌濃度(MIC)及最低殺真菌濃度(MFC);各濃度的CRA分彆作用于BF 48h後, XTT減低法測定生物膜內菌細胞的代謝活力;結晶紫(CV)法定量生物膜。結果受試菌株經過培養24h、48h後可形成穩定的BF。藥物作用48h後,各濃度CRA對菌體代謝活力與空白組相比差異均無統計學意義(P>0.05);較高濃度的CRA組(256、512、1024μg/ml)生物膜量與空白組相比,差異有統計學意義(P<0.05)。結論煙麯黴體外經培養24h、48h後可形成穩定生物膜;金銀花主要活性成分綠原痠不能殺死煙麯黴生物膜細胞,但可以抑製生物膜胞外基質的形成,其抑製作用呈濃度依賴性。
탐토금은화주요활성성분록원산(CRA)대연곡매(A.f)생물막(BF)적체외영향。방법소묘전경(SEM)감정체외연곡매BF;이배희석법측정록원산적최저억균농도(MIC)급최저살진균농도(MFC);각농도적CRA분별작용우BF 48h후, XTT감저법측정생물막내균세포적대사활력;결정자(CV)법정량생물막。결과수시균주경과배양24h、48h후가형성은정적BF。약물작용48h후,각농도CRA대균체대사활력여공백조상비차이균무통계학의의(P>0.05);교고농도적CRA조(256、512、1024μg/ml)생물막량여공백조상비,차이유통계학의의(P<0.05)。결론연곡매체외경배양24h、48h후가형성은정생물막;금은화주요활성성분록원산불능살사연곡매생물막세포,단가이억제생물막포외기질적형성,기억제작용정농도의뢰성。
Objective To explore the effect of the main active component of Honeysuckle (Chlorogenic acid,CRA) on Aspergillus fumigatus (A.f) biofilm (BF) in vitro. Methods The model of A. fumigatus BF was established in vitro and i-dentified by scanning electron microscopy (SEM). The minimum inhibitory concentration (MIC) and the minimum fungicidal concentration (MFC) were measured by double dilution. After affecting 48 hours, the XTT reduction assay was used for the metabolic activity of the fungus inside biofilm. The crystal violet(CV) assay was used for quantification of biofilm. Results BF model was established successfully in vitro after being cultured for 24h and 48h. After affecting 48h , the metabolic activity by XTT assay showed that there was no significant difference among untreated control and CRA groups; there was statistically sig-nificant difference between the biofilm biomass of serially increasing concentrations CRA (256,512,1 024μg/ml) and untreated control (P<0.05). Conclusion Aspergillus fumigatus can form biofilms in vitro after affecting 24h and 48h; the main active component of Honeysuckle(chlorogenic acid) can inhibit the extracellular matrix of BF in vitro,which showed a dose-dependent manner.