mda7-/IL2-4和IL2-4delE5诱导急性髓系白血病细胞向单核细胞分化

目的:研究人黑素瘤分化相关基因-7(melanoma differentiation associated gene-7,mda-7;又称IL-24)及其剪接体IL-24 delE5与急性髓系白血病(acute myeloid leukemia,AML)细胞分化的关系。方法:十四烷酰佛波醇-乙酯(12-O-tetrade-canoylphorbol-13-acetate,TPA)处理人急性髓系白血病细胞系U937、HL-60,real-time PCR及Western blotting检测细胞中mda-7/IL-24和IL-24 delE5的表达,FACS检测细胞表面CD11b、CD14和CD115的表达。siRNA干扰U937、HL-60细胞中mda-7/IL-24和IL-24 delE5的表达后,再以TPA诱导细胞分化,FACS检测CD11b、CD14和CD115的表达。用前期构建的mda-7/IL-24和IL-24 delE5载体转染U937、HL-60及AML-M5患者的原代白血病细胞,观察异位过表达mda-7/IL-24和IL-24 delE5能否诱导白血病细胞向单核细胞分化。结果:TPA在诱导U937、HL-60细胞向单核细胞分化过程中显著促进mda-7/IL-24及其剪接体IL-24 delE5的表达,用siRNA干扰mda-7/IL-24及IL-24 delE5的表达后,TPA诱导U937、HL-60细胞向单核细胞分化的作用也被阻断。异位过表达mda-7/IL-24和IL-24 delE5可诱导U937、HL-60以及原代AML细胞向单核细胞分化:U937、HL-60细胞表面CD11b和CD14表达均显著升高,CD115表达仅在U937细胞有显著升高;3例AML-M5患者的原代AML细胞中CD11b、CD14及CD115表达均有不同程度升高,细胞呈现单核细胞的形态特征。结论:TPA可通过上调mda-7/IL-24及其剪接体IL-24 delE5的表达诱导白血病细胞向单核细胞分化。

携带IL-24的溶瘤腺病毒作用于乳腺癌的体外实验研究

目的构建携带IL-24基因的溶瘤腺病毒CNHK600-IL-24,评估CNHK600-IL-24在体外对乳腺癌细胞的杀伤能力。方法将IL-24基因插入腺病毒穿梭载体SG502-ΔCR2,与5型腺病毒骨架载体pPE3共转染至人胚肾293细胞,获得溶瘤腺病毒CNHK600-IL-24。荧光显微镜观测及病毒体外增殖实验测评病毒在乳腺癌细胞MDA-MB-231和正常成纤维细胞MRC-5中的增殖情况;MTT法检测不同MOI值的病毒对两种细胞的抑制效应;ELISA法检测病毒感染细胞后上清液中IL-24的含量;Western blot法检测细胞内的IL-24蛋白;流式细胞检测细胞的凋亡情况。结果 CNHK600-IL-24经测序及PCR鉴定,病毒滴度为1.9×1010pfu/mL。CNHK600-IL-24感染MDA-MB-231细胞后表现出强大的增殖、复制能力,而在MRC-5细胞内增殖并不明显;CNHK600-IL-24在很低的浓度就能对MDA-MB-231细胞产生明显的杀伤效应,而对MRC-5细胞的杀伤作用明显减弱;CNHK600-IL-24感染MDA-MB-231细胞后,IL-24蛋白的表达明显增多,而感染MRC-5细胞后产生的IL-24维持在很低的水平。流式细胞检测发现,病毒引起的MDA-MB-231细胞明显凋亡而MRC-5细胞的凋亡率很低。结论本研究成功构建高滴度的溶瘤腺病毒CNHK600-IL-24,该病毒具有在乳腺癌细胞中特异性增殖并杀伤肿瘤细胞的能力。

肺炎克雷伯杆菌分泌因子及活菌诱导人肺上皮细胞表达分泌IL-8的研究

目的 :探讨肺炎克雷伯杆菌 (Klebsiellapneumoniae ,Kp)分泌因子及活菌诱导肺上皮细胞株表达和分泌IL 8的状况。方法 :用临床分离株Kp0 3 1 1 6、Kp0 3 1 83的细菌培养上清或活菌刺激肺上皮细胞株A5 49和SPC A 1 ,酶联免疫吸附实验 (ELISA)检测细胞IL 8表达量。结果 :①两株Kp培养上清分别刺激A5 49或SPC A 1后 ,IL 8表达量均有显著增高 (P <0 .0 1 ) ,且随上清刺激浓度增加而上升。②两株Kp及DH5 (活菌分别与SPC A 1共孵育 2h ,用庆大霉素杀死胞外菌 ,继续孵育 2 4h后两株Kp诱导细胞IL 8表达量均显著高于DH5α(P <0 .0 1 ) ,且随细菌数 /细胞数比例增大而上升。结论 :Kp分泌因子及活菌都能够诱导肺上皮细胞IL 8表达 ,而活菌上调IL 8的效应较培育上清分泌因子更显著 ,提示肺上皮细胞在Kp感染刺激的肺部炎症反应中起重要作用。

Enhanced CD19 activity in B cells contributes to immunodeficiency in mice deficient in the ICF syndrome gene Zbtb24

Immunodeficiency,centromeric instability,and facial anomalies(ICF)syndrome is a rare autosomal recessive disorder characterized by DNA hypomethylation and antibody deficiency.It is caused by mutations in DNMT3B,ZBTB24,CDCA7,or HELLS.While progress has been made in elucidating the roles of these genes in regulating DNA methylation,little is known about the pathogenesis of the life-threatening hypogammaglobulinemia phenotype.Here,we show that mice deficient in Zbtb24 in the hematopoietic lineage recapitulate the major clinical features of patients with ICF syndrome.Specifically,Vav-Cre-mediated ablation of Zbtb24 does not affect lymphocyte development but results in reduced plasma cells and low levels of IgM,IgG1,and IgA.Zbtb24-deficient mice are hyper and hypo-responsive to T-dependent and T-independent type 2 antigens,respectively,and marginal zone B-cell activation is impaired.Mechanistically,Zbtb24-deficient B cells show severe loss of DNA methylation in the promoter region of Il5ra(interleukin-5 receptor subunit alpha),and Il5ra derepression leads to elevated CD19 phosphorylation.Heterozygous disruption of Cd19 can revert the hypogammaglobulinemia phenotype of Zbtb24-deficient mice.Our results suggest the potential role of enhanced CD19 activity in immunodeficiency in ICF syndrome.