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胃肠道肽对体外偶氮甲烷处理的结肠黏膜的影响。

Effects of gastrointestinal peptides on azoxymethane-treated colonic mucosa in vitro.

作者信息

Finney K J, Appleton D R, Ince P, Moorghen M, Elliott K, Watson A J

机构信息

Department of Pathology, University of Newcastle upon Tyne, UK.

出版信息

Carcinogenesis. 1991 Nov;12(11):2017-22. doi: 10.1093/carcin/12.11.2017.

Abstract

An organ-culture system has been used to investigate the effect of certain gastrointestinal peptides on the morphology and cell proliferation of explants of azoxymethane (AOM)-treated colonic mucosa. Our aim was to ascertain whether such factors play a direct part in the maintenance of hyperplastic changes in the large intestine. Explants of AOM-treated colonic mucosa from 15 animals were maintained in a serum-free medium in the presence of either gastrin-17 (250 pg/ml and 250 ng/ml), peptide YY (80 pmol/l and 160 pmol/l) epidermal growth factor (EGF) (10 ng/ml and 100 ng/ml) or the C-terminal fragment of glucagon-37 (30 pmol/l) for a period of up to 7 days. Other explants (controls) received fresh medium only each day. After 1, 2, 3, 5 and 7 days of culture both experimental and control explants received vincristine (4 micrograms/ml) for 3 h prior to fixation. The proportion of vincristine-arrested metaphases within the explants was determined together with crypt length. Neither gastrin nor peptide YY was found to influence cell division at either concentration. Despite an initial inhibitory effect, both concentrations of EGF exerted a trophic effect which increased with time. The glucagon-37 fragment caused an immediate increase in proliferation which then declined as time progressed. None of these factors, however, were able to maintain the hyperplastic changes seen in the pre-culture samples of AOM-treated mucosae.

摘要

一种器官培养系统已被用于研究某些胃肠肽对用偶氮甲烷(AOM)处理的结肠黏膜外植体的形态和细胞增殖的影响。我们的目的是确定这些因素是否在大肠增生性变化的维持中起直接作用。从15只动物身上获取经AOM处理的结肠黏膜外植体,将其置于无血清培养基中,分别添加胃泌素-17(250 pg/ml和250 ng/ml)、肽YY(80 pmol/l和160 pmol/l)、表皮生长因子(EGF)(10 ng/ml和100 ng/ml)或胰高血糖素-37的C末端片段(30 pmol/l),培养长达7天。其他外植体(对照组)每天仅接受新鲜培养基。培养1、2、3、5和7天后,实验和对照外植体在固定前3小时接受长春新碱(4微克/毫升)处理。测定外植体内长春新碱阻滞中期的比例以及隐窝长度。未发现胃泌素和肽YY在任何一个浓度下对细胞分裂有影响。尽管EGF的两种浓度最初都有抑制作用,但随后都发挥了营养作用,且随着时间推移而增强。胰高血糖素-37片段使增殖立即增加,但随后随着时间推移而下降。然而,这些因素均无法维持在经AOM处理的黏膜预培养样本中所见的增生性变化。

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