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迪斯帕内阿米巴:与无菌培养的克氏锥虫共培养

Entamoeba dispar: cultivation with sterilized Crithidia fasciculata.

作者信息

Kobayashi S, Imai E, Tachibana H, Fujiwara T, Takeuchi T

机构信息

Department of Tropical Medicine and Parasitology, School of Medicine, Keio University, Tokyo, Japan.

出版信息

J Eukaryot Microbiol. 1998 Mar-Apr;45(2):3S-8S. doi: 10.1111/j.1550-7408.1998.tb04516.x.

Abstract

Four isolates of Entamoeba dispar identified by their hexokinase and phosphoglucomutase isoenzyme profile and by their failure to react with Entamoeba histolytica-specific monoclonal antibody (4G6) could be grown in either Diamond's BI-S-33 medium, newly developed BCSI-S (Biosate cysteine starch iron-serum) medium, or casein-free YI-S medium in the presence of Crithidia fasciculata (ReF-1:PRR) sterilized by heating 56 degrees C for 30 min and subsequent incubation with 1% hydrogen peroxide for 24 hours at 4 degrees C. After the cultures were maintained for over 50 passages, the amebae were identified as E. dispar by isoenzyme analysis, polymerase chain reaction with E. histolytica- and E. dispar-specific primers, i.e. p11 plus p12 and p13 plus p14, respectively, and by negative reactivity with monoclonal antibody 4G6. The flagellates added to the culture were judged to be metabolically inactive based on the results of nuclear magnetic resonance spectroscopy, electron microscopy, and polarographic analysis. All of these findings suggest that E. dispar can grow in vitro with metabolically inactive C. fasciculata as a culture associate.

摘要

通过己糖激酶和磷酸葡萄糖变位酶同工酶谱以及与溶组织内阿米巴特异性单克隆抗体(4G6)不发生反应鉴定出的4株迪斯帕内阿米巴分离株,在存在经56℃加热30分钟灭菌并随后于4℃用1%过氧化氢孵育24小时的 fasciculata(ReF-1:PRR)的情况下,可在戴蒙德氏BI-S-33培养基、新开发的BCSI-S(生物酸盐半胱氨酸淀粉铁-血清)培养基或无酪蛋白的YI-S培养基中生长。在培养物传代50次以上后,通过同工酶分析、分别用溶组织内阿米巴特异性引物和迪斯帕内阿米巴特异性引物(即p11加p12和p13加p14)进行聚合酶链反应以及与单克隆抗体4G6呈阴性反应,将阿米巴鉴定为迪斯帕内阿米巴。根据核磁共振光谱、电子显微镜和极谱分析的结果,判断添加到培养物中的鞭毛虫代谢不活跃。所有这些发现表明,迪斯帕内阿米巴可在体外与代谢不活跃的 fasciculata 作为培养伴生物生长。

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