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人胃上皮细胞单层培养物。

A monolayer culture of human gastric epithelial cells.

作者信息

Terano A, Mach T, Stachura J, Sekhon S, Tarnawski A, Ivey K J

出版信息

Dig Dis Sci. 1983 Jul;28(7):595-603. doi: 10.1007/BF01299919.

Abstract

Our aim was to develop a fibroblast-free monolayer culture of human gastric mucosal cells, using the specimens obtained by routine endoscopic biopsy. Human gastric mucosa obtained from normal volunteers by endoscopic biopsy was dissociated from collagenase and hyaluronidase. Dissociated cells were cultured in supplemented Coon's modified Ham's F-12 medium. Within 24 hr of inoculation, the cells were attached to the culture dishes. This was followed by cellular outgrowth. On phase-contrast microscopy, all cells had epithelial characteristics and fibroblasts were not observed. Ninety percent of cells contained periodic acid Schiff reaction-positive mucous granules after diastase digestion consistent with mucous epithelial cells. Two percent of the cells gave a strong reaction for succinic dehydrogenase activity (parietal cells). Immunohistochemical staining for pepsinogen in cultured cells was negative. On EM, microvilli-like projections, junctional complexes, Golgi apparatus, and mucous granules were apparent in the majority of cells. Mitotic figures were observed by day 3 with Giemsa staining. Autoradiographically, these cells were able to incorporate [3H]TdR into the nuclei. Cells were capable of synthesizing DNA, and this function was inhibited by cycloheximide. Cells could be cultured for up to two weeks without fibroblast contamination. A method of primary monolayer culture of human gastric mucosa obtained by a routine endoscopic biopsy has been successfully developed.

摘要

我们的目标是利用常规内镜活检获取的标本,开发一种无成纤维细胞的人胃黏膜细胞单层培养方法。通过内镜活检从正常志愿者获取的人胃黏膜用胶原酶和透明质酸酶进行解离。解离后的细胞在添加了成分的库恩改良哈姆F-12培养基中培养。接种后24小时内,细胞附着于培养皿。随后细胞开始生长。在相差显微镜下,所有细胞均具有上皮细胞特征,未观察到成纤维细胞。经淀粉酶消化后,90%的细胞含有过碘酸希夫反应阳性的黏液颗粒,符合黏液上皮细胞特征。2%的细胞琥珀酸脱氢酶活性呈强阳性反应(壁细胞)。培养细胞中胃蛋白酶原的免疫组化染色为阴性。在电子显微镜下,大多数细胞可见微绒毛样突起、连接复合体、高尔基体和黏液颗粒。第3天用吉姆萨染色观察到有丝分裂象。通过放射自显影术,这些细胞能够将[3H]胸腺嘧啶核苷掺入细胞核。细胞能够合成DNA,且该功能受环己酰亚胺抑制。细胞可培养长达两周而无成纤维细胞污染。已成功开发出一种通过常规内镜活检获取的人胃黏膜原代单层培养方法。

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