马立克氏病病毒感染鸡TCR1与TCR2T细胞动态变化观察

为深入探讨鸡马立克氏病Ｔ细胞受体亚群的变化与疾病发生与发展的相互关系，本实验以马立克氏病强毒株人工感染１日龄ＳＰＦ雏鸡，在不同的感染期，以流式细胞仪分析脾脏、胸腺、外周血淋巴细胞中ＴＣＲ１＋Ｔ和ＴＣＲ２＋Ｔ细胞的动态变化。结果表明，感染鸡脾脏中ＴＣＲ１＋Ｔ细胞异常增高，而ＴＣＲ２＋Ｔ细胞在脾脏和外周血中表现为暂短的升高，其后迅速下降。

昆虫杆状病毒表达系统表达TCRγ9/δ2-Fc融合蛋白及其生物学功能的初步鉴定

目的建立昆虫杆状病毒表达系统表达TCRγ9/δ2-Fc融合蛋白技术平台并鉴定其表达产物的生物学功能。方法用搭桥PCR获得γ9Fc和δ2(OT3)Fc基因片段,构建成pBACp10ph-γ9/δ2(OT3)-Fc重组质粒,与AcNPV昆虫病毒DNA共转染昆虫sf9细胞,表达TCRγ9/δ2-Fc融合蛋白;Western blot鉴定TCRγ9/δ2-Fc蛋白表达位置;胞内流式细胞仪检测γ9Fc和δ2(OT3)Fc两基因表达效率;蛋白G亲和层析后,SDS-PAGE鉴定蛋白纯度;激光共聚焦扫描显微镜技术和生物传感器技术检测了TCRγ9/δ2-Fc蛋白与SKOV3细胞和MNS蛋白的结合特性。结果成功构建pBACp10ph-γ9/δ2(OT3)-Fc表达载体,经鉴定发现TCRγ9/δ2-Fc蛋白在sf9细胞内表达,但γ9Fc和δ2(OT3)Fc两基因的表达效率有较大差异。纯化得到一定纯度的TCRγ9/δ2-Fc蛋白,并且具有与SKOV3细胞和MNS蛋白结合的特性。结论成功建立昆虫杆状病毒表达系统表达TCRγ9/δ2-Fc融合蛋白的技术平台,表达产物TCRγ9/δ2-Fc可以在体外模拟TCRγδ识别抗原的特性。

共表达TcRα12-2和TCRVβ7.1重组腺病毒载体的构建及其杀伤肝癌细胞作用的研究

目的:构建共表达TCRα12-2和TCRVβ7.1重组腺病毒载体Ad.TCRα12.2-IRES-Vβ7.1,并研究其杀伤肝癌细胞的作用。方法:提取外周血单核细胞(peripheral blood mononuclear cell,PBMC)总RNA,用RT-PCR的方法得到TCRα12-2基因。TCRVβ7.1基因由pCDN3.1-Vβ7.1扩增获得,将这两个基因以IRES相连克隆入腺病毒穿梭质粒pDC315中。穿梭质粒和腺病毒骨架质粒共转染HEK293细胞,包装出可同时表达TCRα12-2和TCRVβ7.1的重组腺病毒。然后提取病毒基因组DNA,对外源目的基因进行PCR鉴定;病毒感染宫颈癌细胞(HELA),48小时后提取细胞总RNA,通过RT-PCR鉴定目的基因表达;最后病毒感染PBMC,用流式细胞仪检测目的蛋白的表达。对鉴定正确的病毒进行大量扩增并测定滴度。用MTT比色法检测Ad.TCRα12-2-IRES-Vβ7.1感染的PBMC对肝癌细胞HEPG2和BEL-7402的杀伤作用。结果:从重组病毒基因组中扩增出目的基因TCRα12-2和TCRVβ7.1,RT-PCR和流式细胞仪检测表明目的基因可以有效的表达。Ad.TCRα12-2-IRES-Vβ7.1感染PBMC组对肿瘤细胞的杀伤率明显高于PBMC组和Ad-GFP感染组。结论:成功构建了双表达TCRα12-2和TCRVβ7.1基因的重组腺病毒载体Ad.TCRα12-2-IRES-Vβ7.1,且其感染后的PBMC可有效的杀伤肝癌细胞。

CDR3δ-grafted γ9δ2T cells mediate effective antitumor reactivity

Adoptive cell-transfer therapy （ACT） has been reported to suppress growing tumors and to overcome tumor escape in animal models. As a candidate ACT effector, γ9δ2T cells can be activated and expanded in vitroand in vivoand display strong antitumor activity against colorectal, lung, prostate, ovarian and renal cell carcinomas. However, it is difficult to obtain a large enough number of γδT cells to meet the need for immunotherapy that can overcome the cancer patients＇ immune suppressive tumor microenvironment. In previous studies, our lab confirmed that γ9δ2T cells recognized tumor cells via the CDR3δ region of the γδ-T-cell receptor （TCR）. We constructed full-length human peripheral blood mononuclear cell （PBMC）-derived γ9 and δ2 chains in which the CDR3 region was replaced by an ovarian epithelial carcinoma （OEC）-derived CDR3. We transferred the CDR3δ-grafted γ9δ2TCR into peripheral blood lymphocytes （PBLs） to develop genetically modified γ9δ2T cells. In vitro studies have shown that these CDR3δ-grafted γ9δ2T cells can produce cytokines after stimulation with tumor cell extracts and exhibit cytotoxicity towards tumor cells, including human OEC and cervical adenocarcinoma. CDR3δ-grafted γ9δ2T cells adoptively transferred into nude mice bearing a human OEC cell line demonstrated significant antitumor effects. These results indicate that CDR3δ-grafted γ9δ2T cells might be candidates for clinical tumor immunotherapy.