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在体内研究大鼠结肠腔和黏液层中的溶组织内阿米巴滋养体。

Entamoeba histolytica trophozoites in the lumen and mucus blanket of rat colons studied in vivo.

作者信息

Leitch G J, Dickey A D, Udezulu I A, Bailey G B

出版信息

Infect Immun. 1985 Jan;47(1):68-73. doi: 10.1128/iai.47.1.68-73.1985.

Abstract

Trophozoites of Entamoeba histolytica HM-1 were cultivated axenically in TYI-S medium. The amoebae were then transferred into this medium lacking serum (TYI) and inoculated into in vivo colon loops of adult Sprague-Dawley rats. The trophozoites were rapidly absorbed by the mucus, and few were found free in the luminal fluid by 1 h. By 4 h, the amoebae began to reappear in the lumen, aggregated in sloughed mucus blanket fragments. The colon was examined histologically and by scanning electron microscopy. There was no evidence of invasion or even brush-border attachment by the trophozoites within 4 h. In TYI, trophozoite motility was low. Exposure to the colonic lumen environment for 5 min in this medium significantly increased motility. However, as the trophozoites became absorbed to mucus fragments, their observed motility virtually ceased despite some morphological evidence of pseudopod extension. Erythrophagocytosis was not significantly affected by either exposing trophozoites to TYI washings of the colonic lumen, or by the more complete medium, TYI-S, in which the amoebae were significantly more motile. Two major mucus glycoprotein oligosaccharide end-group sugars, L-fucose and N-acetyl-neuraminic acid, were tested for their effects on trophozoite motility in both TYI and TYI-S. L-Fucose reduced motility; the sialic acid increased motility. It is concluded that the intestinal lumen contains several compartments, including the luminal fluid and the mucus blanket, and that Entamoeba trophozoites exist in a highly motile state in the former and a low motility state in the latter. The mucus blanket provided a significant barrier to trophozoite access to intestinal epithelium target tissue.

摘要

溶组织内阿米巴HM-1滋养体在TYI-S培养基中进行无菌培养。然后将这些阿米巴转移到不含血清的该培养基(TYI)中,并接种到成年Sprague-Dawley大鼠的体内结肠肠袢中。滋养体迅速被黏液吸收,1小时后在管腔液中几乎未发现游离的滋养体。4小时后,阿米巴开始重新出现在肠腔中,聚集在脱落的黏液毯碎片中。对结肠进行组织学检查和扫描电子显微镜检查。4小时内没有证据表明滋养体有侵袭甚至刷状缘附着现象。在TYI中,滋养体的运动性较低。在该培养基中暴露于结肠肠腔环境5分钟可显著增加运动性。然而,随着滋养体被黏液碎片吸收,尽管有一些伪足延伸的形态学证据,但观察到的运动性实际上停止了。无论是将滋养体暴露于结肠肠腔的TYI冲洗液中,还是在阿米巴运动性明显更高的更完整培养基TYI-S中,吞噬红细胞现象均未受到显著影响。测试了两种主要的黏液糖蛋白寡糖末端基团糖,L-岩藻糖和N-乙酰神经氨酸,对它们在TYI和TYI-S中对滋养体运动性的影响。L-岩藻糖降低运动性;唾液酸增加运动性。得出的结论是,肠腔包含几个区域,包括管腔液和黏液毯,并且溶组织内阿米巴滋养体在前一种区域中以高运动状态存在,而在后一种区域中以低运动状态存在。黏液毯为滋养体进入肠上皮靶组织提供了显著的屏障。

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