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大鼠肝脏核仁110S及总核糖核蛋白颗粒的蛋白质成分研究

Studies on the protein components of 110S and total ribonucleoprotein particles of rat liver nucleoli.

作者信息

Fujisawa T, Imai K, Tanaka Y, Ogata K

出版信息

J Biochem. 1979 Jan;85(1):277-86. doi: 10.1093/oxfordjournals.jbchem.a132321.

Abstract

Proteins of rat liver nucleolar RNP, especially 110S RNP containing 45S RNA, were investigated and the following results were obtained. 1. Nucleolar extract was prepared from thioacetamide-treated rat liver nucleoli in the presence of 1 mg PVS per ml. Sucrose-density gradient centrifugation of the nucleolar extract showed RNP distributed between 60S and 110S. The 110S particles (110S RNP) contain 45S RNA as judged from the radioactivity profiles of nucleolar extract labelled in vivo with [3H]orotic acid for 10 min and 2 h. The protein components of 110S RNP and total RNP heavier than 60S (total RNP) were analyzed and compared. 2. Since the effects of PVS treatment on the extraction and the electrophoretic pattern of ribosomal proteins were removed by increasing the Mg2+ concentration during acetic acid extraction, as described in our preceding paper (1), proteins of 110S RNP as well as total RNP from PVS-pretreated nucleoli were extracted with 67% acetic acid containing 334 mM Mg2+ and analyzed by two-dimensional acrylamide gel electrophoresis. Ribosomal proteins masked by contaminating histone spots on the gel were identified by SDS-acrylamide gel electrophoresis. 3. 110S RNP contained a large portion of ribosomal proteins from large subunits; 24 protein spots were distinct, 6 protein spots were faint and 5 proteins (L3, L8, L30, L35, and L36) were missing completely. On the other hand, 110S RNP contained a small number of small subunit proteins; only 6 proteins showed distinct spots, 7 proteins showed faint spots and 12 protein spots were missing. 110S particles contained 11 non-ribosomal proteins, although it is difficult to rule out the possibility that some of them were contaminating chromatin proteins. 4. Total RNP showed electrophoretic patterns of 60S ribosomal proteins similar to those of 110S RNP, although L3 protein was present as a faint spot and 26 proteins showed distinct spots. Total RNP contained more small subunit proteins than 110S RNP; 7 proteins spots were distinct, 10 protein spots were faint and 8 protein spots were missing. The results suggest that some kinds of 40S proteins and L3 protein are attached to 110S RNP during the processing of 110S RNP.

摘要

对大鼠肝脏核仁核糖核蛋白(RNP)的蛋白质,特别是含有45S RNA的110S RNP进行了研究,并获得了以下结果。1. 在每毫升含有1毫克聚乙烯亚硫酸酯(PVS)的条件下,从硫代乙酰胺处理的大鼠肝脏核仁中制备核仁提取物。对核仁提取物进行蔗糖密度梯度离心,结果显示RNP分布在60S至110S之间。根据用[3H]乳清酸在体内标记10分钟和2小时的核仁提取物的放射性图谱判断,110S颗粒(110S RNP)含有45S RNA。对110S RNP和比60S重的总RNP(总RNP)的蛋白质成分进行了分析和比较。2. 如我们前文(1)所述,由于在乙酸提取过程中增加Mg2+浓度可消除PVS处理对核糖体蛋白质提取和电泳图谱的影响,因此用含有334 mM Mg2+的67%乙酸提取PVS预处理核仁中的110S RNP以及总RNP,并通过二维聚丙烯酰胺凝胶电泳进行分析。通过SDS - 聚丙烯酰胺凝胶电泳鉴定凝胶上被污染的组蛋白斑点掩盖的核糖体蛋白质。3. 110S RNP包含来自大亚基的大部分核糖体蛋白质;24个蛋白斑点清晰,6个蛋白斑点模糊,5种蛋白质(L3、L8、L30、L35和L36)完全缺失。另一方面,110S RNP包含少量小亚基蛋白质;只有6种蛋白质显示出清晰的斑点,7种蛋白质显示出模糊的斑点,12个蛋白斑点缺失。110S颗粒包含11种非核糖体蛋白质,尽管难以排除其中一些是污染的染色质蛋白质的可能性。4. 总RNP显示出与110S RNP相似的60S核糖体蛋白质的电泳图谱,尽管L3蛋白以模糊斑点形式存在,26种蛋白质显示出清晰的斑点。总RNP比110S RNP含有更多的小亚基蛋白质;7个蛋白斑点清晰,10个蛋白斑点模糊,8个蛋白斑点缺失。结果表明,在110S RNP的加工过程中,某些种类的40S蛋白质和L3蛋白附着于110S RNP。

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