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一种利用表达绿色荧光蛋白的重组卡介苗监测牛分枝杆菌卡介苗运输的新方法。

A novel method for monitoring Mycobacterium bovis BCG trafficking with recombinant BCG expressing green fluorescent protein.

作者信息

Luo Y, Szilvasi A, Chen X, DeWolf W C, O'Donnell M A

机构信息

Division of Urology, Beth Israel Hospital, Harvard Medical School, Massachusetts 02215, USA.

出版信息

Clin Diagn Lab Immunol. 1996 Nov;3(6):761-8. doi: 10.1128/cdli.3.6.761-768.1996.

DOI:10.1128/cdli.3.6.761-768.1996
PMID:8914772
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC170444/
Abstract

To better understand intracellular and extracellular trafficking of Mycobacterium bovis bacillus Calmette-Guérin (BCG) when used as an intravesical agent in the treatment of transitional cell carcinoma (TCC) of the bladder, recombinant BCG (rBCG) expressing the jellyfish green fluorescent protein (GFP) was created. When the MB49.1 murine TCC cell line was incubated with GFP-expressing rBCG, internalization of the pathogen could be directly visualized by UV microscopy and quantitated by flow cytometry. The in vitro internalization of the GFP rBCG by the bladder tumor cells was temperature dependent, occurring most readily at 37 degrees C and being severely inhibited at 4 degrees C. Optimum internalization was achieved in vitro at a 10:1 BCG-to-tumor cell ratio over 24 h during which approximately 16% of the tumor cells became infected. Cytochalasin B, a phagocytosis inhibitor, abrogated the ingestion by almost 100% at a concentration of 200 micrograms/ml, indicating that contractile microfilaments likely played an important role in this process. By using mitomycin, a DNA cross-linking reagent, to inhibit proliferation of MB49.1 cells, clearance of about 40% of the green rBCG was achieved by 3 days postinfection. No significant difference between the GFP rBCG and wild-type BCG was observed in the ability to induce the expression of cell membrane proteins of major histocompatibility classes I and II, ICAM-I and -II, B7-1 and -2, of Fas from MB49.1 cells or cytokine production from mouse spleen cells. These results indicate that GFP rBCG may serve as a useful substitute for wild-type BCG in future studies of in vivo trafficking experimental and clinical immunotherapy.

摘要

为了更好地理解卡介苗(BCG)作为膀胱内用药治疗膀胱移行细胞癌(TCC)时在细胞内和细胞外的转运情况,构建了表达水母绿色荧光蛋白(GFP)的重组卡介苗(rBCG)。当将MB49.1小鼠TCC细胞系与表达GFP的rBCG共同孵育时,可通过紫外线显微镜直接观察到病原体的内化,并通过流式细胞术进行定量分析。膀胱肿瘤细胞对GFP rBCG的体外内化具有温度依赖性,在37℃时最容易发生,而在4℃时受到严重抑制。在体外,当BCG与肿瘤细胞的比例为10:1、孵育24小时时可实现最佳内化,在此期间约16%的肿瘤细胞被感染。吞噬作用抑制剂细胞松弛素B在浓度为200微克/毫升时可使摄取几乎完全消除,这表明收缩性微丝可能在此过程中起重要作用。通过使用DNA交联剂丝裂霉素抑制MB49.1细胞的增殖,感染后3天可清除约40%的绿色rBCG。在诱导MB49.1细胞主要组织相容性I类和II类细胞膜蛋白、ICAM-I和-II、B7-1和-2以及Fas的表达或小鼠脾细胞产生细胞因子的能力方面,未观察到GFP rBCG与野生型BCG之间存在显著差异。这些结果表明,在未来体内转运实验和临床免疫治疗的研究中,GFP rBCG可能是野生型BCG的有用替代品。