小鼠原发性胆汁性肝硬化与调节T细胞的相关性

目的研究原发性胆汁性肝硬化(primary biliary cirrhosis,PBC)小鼠模型中调节T细胞(regulatory T cell,Treg)及其重要的调节因子转化生长因子β1(transforming growth factor-β1,TGF-β1)与发病的关系以及二者之间的关系。方法选取第8、16、24周PBC小鼠模型及正常对照小鼠(每组6只)-80℃冻存血清,使用酶联免疫吸附分析(enzyme-linked immunosorbent assay,ELISA)法测定血清TGF-β1含量;选取各组小鼠-80℃冻存肝脏标本,使用免疫印迹法半定量测定FOXP3含量;选取各组小鼠常温保存肝脏石蜡标本,使用免疫组化法标记FOXP3+Treg细胞,对汇管区淋巴细胞及FOXP3+Treg进行细胞计数。结果除16周PBC小鼠与24周PBC小鼠血清中TGF-β1含量存在统计学差异(0.174±0.084 vs.0.285±0.080,P=0.041)外,其他各组小鼠之间(包括8、16、24周PBC小鼠与正常对照比较)均无统计学差异;各组小鼠肝脏中均未测出FOXP3蛋白;根据PBC患者分期,PBC小鼠模型分期主要在1期和2期;各组PBC小鼠汇管区淋巴细胞数与同时期正常对照组相比,差异均具有显著统计意义(8周:394 vs.8,P=0.004,16周:392 vs.19,P=0.000,24周:171vs.18,P=0.000),且24周PBC小鼠汇管区淋巴细胞数显著低于16周PBC小鼠(171 vs.392,P=0.006);16、24周PBC小鼠Treg细胞数目显著高于同时期正常对照小鼠(11 vs.0,11 vs.0,P值分别为0.032,0.032)。结论 24周左右PBC小鼠肝脏病变进入纤维化阶段,同时期外周TGF-β1增高,肝脏组织Treg细胞数目增多;TGF-β1及Treg细胞与PBC肝纤维化有关,TGF-β1可能对Treg细胞的增生起促进作用。

蜱抗原诱导的宿主免疫力的研究

报道在实验室控制条件下，用二棘血啤叮咬家兔诱导其产生获得性免疫力。结果表示：叮咬组家兔经ELISA法测定其体内抗（OD值0．54），较对照组（OD值0．09）有显著升高（P＜0．01），叮咬家兔后其^3H-TdR淋巴细胞转化试验的PHA刺激指数为67．11±35．16，较对照组15．49±14．53，有显著升高（P＜0．01），另外，两组的皮肤试验也有极显著差异。（P＜0．001），表明家兔对二棘血蜱咬所产生的获得性免疫力不仅与宿主的体液免疫有关，同时也与宿主的细胞免疫有关。

短波紫外线照射对T淋巴细胞的影响

用136mJ/cm^2短波紫外线照射小鼠,T细胞转化受抑制,抑制率为56％,此作用照射后12小时最为明显,36小时恢复正常。同等剂量照射下对T辅助细胞产生白介素2及胸腺细胞自发增殖无显著性影响。用特大剂量1085mJ/cm^2照射,T细胞转化无显著变化。

Transplantation of human hepatocytes into tolerized genetically immunocompetent rats

AIM: To determine whether normal genetically immunocompetent rodent hosts could be manipulated to accept human hepatocyte transplants with long term survival without immunosuppression. METHODS: Tolerance towards human hepatocytes was established by injection of primary human hepatocytes or Huh7 human hepatoma cells into the peritoneal cavities of fetal rats. Corresponding cells were subsequently transplanted into newborn rats via intrasplenic injection within 24h after birth. RESULTS: Mixed lymphocyte assays showed that spleen cells from non-tolerized rats were stimulated to proliferate when exposed to human hepatocytes, while cells from tolerized rats were not. Injections made between 15 d and 17 d of gestation produced optimal tolerization. Transplanted human hepatocytes in rat livers were visualized by immunohistochemical staining of human albumin. By dot blotting of genomic DNA in livers of tolerized rats 16 weeks after hepatocyte transplantation, it was found that approximately 2.5 X 10(5) human hepatocytes survived per rat liver. Human albumin mRNA was detected in rat livers by RT-PCR for 15 wk, and human albumin protein was also detectable in rat serum. CONCLUSION: Tolerization of an immuno-competent rat can permit transplantation, and survival of functional human hepatocytes.

Hepatitis E virus chimeric DNA vaccine elicits immunologic response in mice

AIM： To construct the plasmid pcHEV23 containing fragments of HEV ORF2 and ORF3 chimeric gene and to assess its ability to elicit specific immunologic response in mice. METHODS： The gene encoding the structural protein of HEV ORF2 fragment and full-length ORF3 was amplified by PCR. The PCR products were cloned into an eucaryotic expression plasmid pcDNA3. The resulting plasmid pcHEV23 was used as a DNA vaccine to inoculate BALB/c mice intramuscularly thrice at a dose of 100 or 200 ug. Mice injected with empty pcDNA3 DNA or saline served as control and then specific immune responses in the mice were detected. RESULTS： After 2-3 times of inoculation, all mice injected with pcHEV23 had anti-HEV IgG seroconversion and specific T lymphocyte proliferation. The lymphocyte stimulation index in the group immunized with pcHEV23 （3.1＋0.49） was higher than that in the control group （0.787±0.12, P〈0.01）. None in the control group had a detectable level of anti-HEV IgG. CONCLUSION： DNA vaccine containing HEV ORF2 and ORF3 chimeric gene can successfully induce specific humoral and cellular immune response in mice.