目的 探讨树突状细胞(DC)与黑色素瘤细胞(B16)体外共培养后对小鼠黑色素瘤生长的影响.方法 提取小鼠骨髓细胞,分化DC,培养至第6天,将细胞分为4组,脂多糖(LPS)组、聚肌胞[Poly(IC)]组、Melan-A抗原肽(Melan-A)组分别加入DC佐剂LPS(终浓度100 ng/mL)、Poly(IC)(终浓度20 ng/mL)、Melan-A抗原肽(终浓度5μmol/L)进行处理,未处理组未进行干预.采用流式细胞术检测DC成熟状态.B16细胞与培养第6天的DC共培养2 d.取C57BL/6J小鼠皮下注射B16细胞(8只),DC+B16细胞(8只),LPS(8只)、poly(IC)(8只)、Melan-A抗原肽激活(8只)的DC+B16细胞,接种B16细胞1周再接种DC+B16细胞(5只),对照组(3只)不接种细胞.于接种第14天取部分小鼠处死,取脾脏,镜下观察其组织形态,接种第28天测算肿瘤体积.结果 LPS组、Poly(IC)组、Melan-A组成熟DC多于未处理组.接种DC+B16细胞的小鼠未见肿瘤生长;接种第28天,与接种B16细胞的小鼠比较,接种LPS、poly(IC)、Melan-A抗原肽激活的DC+B16细胞及接种B16细胞1周再接种DC+B16细胞的小鼠肿瘤体积减小(P均<0.05).与对照组比较,第14天接种DC+B16细胞小鼠脾脏滤泡结构无明显变化,而接种B16细胞及LPS、poly(IC)、Melan-A抗原肽激活的DC+B16细胞小鼠,脾脏滤泡结构增加.结论 DC与B16共培养的可抑制小鼠黑色素瘤的形成.%Objective To investigate the effect of co-culturing dendritic cells (DC)with melanoma cells (B16)on growth of melanoma in mice.Methods We extracted the bone marrow cells.Mouse DC were cultured for 6 days and then were divided into 4 groups:lipopolysaccharide (LPS)group,Poly (IC)group,Melan-A group and the control group. Cells in the LPS group,Poly (IC)group,Melan-A group were incubated with LPS (LPS with final concentration of 100 ng/mL),poly-inosinic-cytidylic acid [Poly(IC)with final concentration of 20 ng/mL]and Melan-A peptide (with final concentration of 5 μmol/L),respectively.The control group was not treated.Flow cytometry was used to study the matura-tion and activation state of DC.B16-F10 (B16)melanoma cells were co-cultured with DC for 2 days and then were used for inoculation of mice.For melanoma model,C57BL/6J mice were inoculated subcutaneously.Some mice were killed at 14 days after inoculation and their spleens were taken to study the structural changes by histochemistry.Tumor size was meas-ured at 28 days after inoculation.Results More mature DC were produced after LPS,Poly(IC)or Melan-A peptide treat-ment as compared with that of the control group (P <0.05).There was no tumor growth after DC +B16 cell inoculation. Compared with the mice inoculated with B16 cells only,the tumor volume was smaller in the mice inoculated with LPS,Po-ly(IC)or Melan-A peptide-activated DC +B16 cells or the mice inoculated with B16 cells one week later followed by an-other inoculation of DC +B16 cells (all P <0.05).Compared with the control group,there was no structural change of the spleen follicles in the mice inoculated with DC +B16,but the number of spleen follicles was increased in the mice inocula-ted with B16 or with LPS,Poly (IC),or Melan-A peptide-activated DC +B16 cells.Conclusion DC co-cultured with B16 can inhibit the growth of melanoma in mice.
展开▼
