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人结肠癌细胞系生长因子的产生

Growth factor production by human colon carcinoma cell lines.

作者信息

Anzano M A, Rieman D, Prichett W, Bowen-Pope D F, Greig R

机构信息

Department of Cell Biology, Smith Kline & French Laboratories, King of Prussia, Pennsylvania 19406.

出版信息

Cancer Res. 1989 Jun 1;49(11):2898-904.

PMID:2541895
Abstract

Conditioned media collected under serum-free conditions over 24 to 48 h from 18 human colon adenocarcinoma cell lines were analyzed for transforming growth factor, types alpha and beta (TGF-alpha and -beta), and platelet-derived growth factor in assays for anchorage-independent growth and radioreceptor competition. Detectable levels of TGF-alpha, TGF-beta, and platelet-derived growth factor were produced by 17, 16, and 6 cell lines, respectively. Three liters of conditioned medium from highly tumorigenic (HT-29, DLD-1, and SW620) and nontumorigenic (SKCO-1) colon cell lines and from nonneoplastic rat kidney (NRK-52E) and small intestinal (IEC-6) epithelial cells were purified by high-performance liquid chromatography and assayed for TGF-alpha- and TGF-beta-like activity. The highly tumorigenic colon cell lines produced 10- to 45-fold (soft agar), 19- to 90-fold (radioreceptor), and 4- to 35-fold (radioimmunoassay) more TGF-alpha activity compared to the nonneoplastic rat intestinal (IEC) epithelial cells. NRK-52E did not produce detectable TGF-alpha activity. Radioimmunoassay analysis of peak fractions revealed only TGF-alpha immunoreactivity; epidermal growth factor was not detected. Levels of TGF-beta-like material in the colon carcinoma populations were comparable (HT-29) or elevated (DLD-1, SW620) only 3- to 4-fold (soft agar) or 1- to 3-fold (radioreceptor binding) compared to IEC cells or NRK-52E. Growth factor production is an ubiquitous property of colon carcinoma cell lines maintained in vitro and is consistent with this class of molecule, playing a contributory role in regulating cell growth.

摘要

在无血清条件下,从18个人类结肠腺癌细胞系中收集24至48小时的条件培养基,分析其转化生长因子α和β(TGF-α和 -β)以及血小板衍生生长因子,用于非锚定依赖性生长和放射受体竞争分析。分别有17、16和6个细胞系产生了可检测水平的TGF-α、TGF-β和血小板衍生生长因子。从高致瘤性(HT-29、DLD-1和SW620)和非致瘤性(SKCO-1)结肠细胞系以及非肿瘤性大鼠肾(NRK-52E)和小肠(IEC-6)上皮细胞中收集的3升条件培养基,通过高效液相色谱法进行纯化,并检测其TGF-α和TGF-β样活性。与非肿瘤性大鼠肠(IEC)上皮细胞相比,高致瘤性结肠细胞系产生的TGF-α活性在软琼脂分析中高10至45倍、放射受体分析中高19至90倍、放射免疫分析中高4至35倍。NRK-52E未产生可检测到的TGF-α活性。对峰馏分的放射免疫分析仅显示TGF-α免疫反应性;未检测到表皮生长因子。与IEC细胞或NRK-52E相比,结肠癌细胞群体中TGF-β样物质的水平仅在软琼脂分析中升高3至4倍、放射受体结合分析中升高1至3倍(HT-29)或更高(DLD-1、SW620)。生长因子的产生是体外培养的结肠癌细胞系的普遍特性,并且与这类分子一致,在调节细胞生长中起促进作用。

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