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通过多聚核糖体相关mRNA体外合成蛋白质来检测人原代淋巴细胞激活过程中的早期基因表达变化。

Detection of early gene expression changes during activation of human primary lymphocytes by in vitro synthesis of proteins from polysome-associated mRNAs.

作者信息

Miyamoto S, Qin J, Safer B

机构信息

Molecular Hematology Branch, Section on Protein and RNA Biosynthesis, National Heart, Lung, and Blood Institute, National Institutes of Health, Bethesda, Maryland 20892, USA.

出版信息

Protein Sci. 2001 Feb;10(2):423-33. doi: 10.1110/ps.21301.

DOI:10.1110/ps.21301
PMID:11266628
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2373944/
Abstract

The rapid increase in protein synthesis during the mitogenic stimulation of human peripheral blood lymphocyte is the result of global and specific translational control mechanisms. To study some of these mechanisms, we examined the in vitro translatability of mRNAs associated with the polyribosome fraction. Polyribosome fractions were isolated from lymphocytes after activation with ionomycin and the phorbol ester PMA. The associated PAmRNAs were translated in the presence of mRNA-depleted rabbit reticulocyte lysate and [(35)S]Met, and the protein products were analyzed by SDS--PAGE and autoradiography. There was little synthesis of protein from the PAmRNAs isolated from unactivated T cells, but the PAmRNAs isolated from activated T cells showed a rapid increase in translatability. Translation of the PAmRNAs was sensitive to edeine and m7GTP, suggesting their cap-dependent translation. With activation, the majority of proteins showed increasing in vitro translation, but two proteins, p72 and p33, were found to have increased synthesis within 30 min, which decreased in 1 h. Transcription inhibitors were used to ascertain if regulation of their expression was transcriptional or translational. To identify these proteins, we used biotinylated lysine during the in vitro translation reaction, and we extracted the biotinylated protein by using streptavidin magnetic beads. The protein product was analyzed by mass spectrometry. p33 was identified as a prohibitin-like protein (BAP37), but the identification of p72 was not found in the databases. The distinct up-regulation and down-regulation of their protein expression suggest their tightly controlled regulation during early T cell activation.

摘要

人外周血淋巴细胞在有丝分裂原刺激下蛋白质合成的快速增加是全局和特定翻译控制机制的结果。为了研究其中一些机制,我们检测了与多核糖体部分相关的mRNA的体外可翻译性。在用离子霉素和佛波酯PMA激活后,从淋巴细胞中分离多核糖体部分。相关的PAmRNA在缺乏mRNA的兔网织红细胞裂解物和[(35)S]甲硫氨酸存在下进行翻译,蛋白质产物通过SDS-PAGE和放射自显影进行分析。从未激活的T细胞中分离的PAmRNA几乎没有蛋白质合成,但从激活的T细胞中分离的PAmRNA显示出可翻译性的快速增加。PAmRNA的翻译对依地尼和m7GTP敏感,表明它们依赖帽依赖性翻译。随着激活,大多数蛋白质显示出体外翻译增加,但发现两种蛋白质p72和p33在30分钟内合成增加,在1小时内减少。使用转录抑制剂来确定它们的表达调控是转录性的还是翻译性的。为了鉴定这些蛋白质,我们在体外翻译反应中使用了生物素化的赖氨酸,并使用链霉亲和素磁珠提取生物素化的蛋白质。通过质谱分析蛋白质产物。p33被鉴定为一种类禁止素蛋白(BAP37),但在数据库中未找到p72的鉴定结果。它们蛋白质表达的明显上调和下调表明它们在早期T细胞激活过程中受到严格控制。

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