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培养的大鼠Ⅱ型肺细胞中表皮生长因子的转录、翻译及信号转导

Epidermal growth factor transcription, translation, and signal transduction by rat type II pneumocytes in culture.

作者信息

Raaberg L, Nexø E, Buckley S, Luo W, Snead M L, Warburton D

机构信息

Division of Neonatology and Pediatric Pulmonology, Childrens Hospital of Los Angeles, CA 90027.

出版信息

Am J Respir Cell Mol Biol. 1992 Jan;6(1):44-9. doi: 10.1165/ajrcmb/6.1.44.

Abstract

Epidermal growth factor (EGF) is known to induce fetal lung maturation and its receptor is present in the lungs of several species. Recently, EGF has been immunolocalized in type II pneumocytes in rat lung. We postulated that EGF is synthesized in type II pneumocytes and that, because of its position-restricted distribution within the alveolus, EGF might act as an autocrine regulator of type II pneumocyte function. Herein, we have tested the hypothesis using adult rat type II pneumocytes in primary culture. In situ hybridization, using an oligonucleotide probe corresponding to amino acid residues 1070 to 1081 of mouse EGF precursor, demonstrated the presence of EGF precursor mRNA. Upon S-200 Sephacryl gel chromatography of type II pneumocyte extracts, EGF-reactive protein eluted as a high-molecular-weight form (greater than 100 kD). EGF immunoreactivity was localized within type II pneumocytes in the periphery of groups of 10 to 15 cells in culture. The type II pneumocytes bound [125I]EGF in a specific manner, indicating the presence of EGF receptors. Scatchard plots gave an apparent affinity constant (Ka) of 1 x 10(9) liters/mol, and the number of receptors was estimated to be 4.8 x 10(11) mg protein (50 per cell). EGF receptor binding specificity was confirmed by the absence of an autoradiographic signal for cells incubated in the presence of a 100-fold excess concentration of transforming growth factor-alpha. Binding of [125I]EGF could also be downregulated 95% by incubation with 0.2 nM transforming growth factor-alpha.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

表皮生长因子(EGF)已知可诱导胎儿肺成熟,其受体存在于多种物种的肺中。最近,EGF已在大鼠肺的II型肺细胞中进行了免疫定位。我们推测EGF在II型肺细胞中合成,并且由于其在肺泡内的位置受限分布,EGF可能作为II型肺细胞功能的自分泌调节剂。在此,我们使用原代培养的成年大鼠II型肺细胞对这一假设进行了测试。使用与小鼠EGF前体氨基酸残基1070至1081相对应的寡核苷酸探针进行原位杂交,证明了EGF前体mRNA的存在。对II型肺细胞提取物进行S-200 Sephacryl凝胶色谱分析时,EGF反应性蛋白以高分子量形式(大于100 kD)洗脱。在培养的10至15个细胞组周边的II型肺细胞中检测到EGF免疫反应性。II型肺细胞以特异性方式结合[125I]EGF,表明存在EGF受体。Scatchard图给出的表观亲和常数(Ka)为1×10⁹升/摩尔,受体数量估计为4.8×10¹¹/毫克蛋白(每个细胞50个)。在100倍过量浓度的转化生长因子-α存在下孵育的细胞,其放射自显影信号缺失,证实了EGF受体结合的特异性。用0.2 nM转化生长因子-α孵育也可使[125I]EGF的结合下调95%。(摘要截短于250字)

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