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兔结肠和人直肠黏膜活检组织中糖蛋白的合成与分泌

Glycoprotein synthesis and secretion by mucosal biopsies of rabbit colon and human rectum.

作者信息

MacDermott R P, Donaldson R M, Trier J S

出版信息

J Clin Invest. 1974 Sep;54(3):545-54. doi: 10.1172/JCI107791.

DOI:10.1172/JCI107791
PMID:4852174
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC301587/
Abstract

Elucidation of mechanisms involved in the control of colonic production of mucus requires direct examination of glycoprotein synthesis and secretion by colonic mucosa. In the past, the limited viability of intestinal mucosa in vitro has hampered such investigations. When maintained in an organ culture system, mucosal biopsies of rabbit colon and human rectum remained viable for 24 h as documented by morphologic appearance and a steady rate of protein synthesis and secretion. These biopsies also incorporated (14)C-labeled glucosamine into tissue glycoproteins and secreted labeled glycoproteins at a steady rate for 24 h. Glucosamine was predominantly incorporated into macromolecules that were ultimately secreted, in contrast to leucine, which was predominantly incorporated into tissue macromolecules. When studied by autoradiography, cultured rabbit colonic biopsies synthesized and secreted glycoproteins in vitro at cellular sites and over a time-course similar to those previously described for the intestine of intact animals. Acetylcholine consistently stimulated secretion of labeled glycoproteins but did not alter glycoprotein synthesis. In contrast, cycloheximide inhibited glycoprotein synthesis but had no effect on the secretion of newly synthesized glycoproteins. Rectal biopsies from patients with active ulcerative colitis incorporated increased amounts of [(14)C]glucosamine into glycoproteins during organ culture and secreted labeled glycoproteins more rapidly into the incubation medium when compared to biopsies obtained from healthy volunteers These findings indicate that organ culture provides a useful means of directly examining the synthesis and secretion of glycoproteins by healthy and diseased colonic mucosa.

摘要

阐明参与控制结肠黏液产生的机制需要直接检测结肠黏膜中糖蛋白的合成和分泌。过去,肠黏膜在体外有限的存活能力阻碍了此类研究。当维持在器官培养系统中时,兔结肠和人直肠的黏膜活检标本在24小时内保持存活,这通过形态学外观以及蛋白质合成和分泌的稳定速率得以证明。这些活检标本还将(14)C标记的葡糖胺掺入组织糖蛋白中,并以稳定的速率分泌标记的糖蛋白达24小时。与亮氨酸主要掺入组织大分子不同,葡糖胺主要掺入最终被分泌的大分子中。当通过放射自显影研究时,培养的兔结肠活检标本在体外合成和分泌糖蛋白的细胞位点及时程与先前描述的完整动物肠道相似。乙酰胆碱持续刺激标记糖蛋白的分泌,但不改变糖蛋白的合成。相反,环己酰亚胺抑制糖蛋白的合成,但对新合成糖蛋白的分泌没有影响。与从健康志愿者获得的活检标本相比,活动期溃疡性结肠炎患者的直肠活检标本在器官培养期间将更多量的[(14)C]葡糖胺掺入糖蛋白中,并将标记的糖蛋白更快地分泌到培养液中。这些发现表明,器官培养为直接检测健康和患病结肠黏膜中糖蛋白的合成和分泌提供了一种有用的方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b005/301587/f7cb4751cad5/jcinvest00161-0055-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b005/301587/f7cb4751cad5/jcinvest00161-0055-a.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b005/301587/f7cb4751cad5/jcinvest00161-0055-a.jpg

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