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丝裂原激活的牛淋巴细胞中蛋白质合成的调控。肌动蛋白特异性和总mRNA积累与利用的分析。

Regulation of protein synthesis in mitogen-activated bovine lymphocytes. Analysis of actin-specific and total mRNA accumulation and utilization.

作者信息

Degen J L, Neubauer M G, Degen S J, Seyfried C E, Morris D R

出版信息

J Biol Chem. 1983 Oct 25;258(20):12153-62.

PMID:6195151
Abstract

In response to the mitogenic lectin concanavalin A, the rate of protein synthesis in bovine small lymphocytes increased about 3-fold in 10 h and about 6-fold in 24 h. The rate of synthesis of the cytoskeletal protein actin, which comprises about 10% of total protein synthesis, increased in parallel with total protein synthesis. The cellular levels of actin mRNA were determined at various times after mitogen addition using a cDNA probe derived from a recombinant plasmid carrying a fragment coding for bovine actin. Actin mRNA sequences were found to increase significantly within 3 h and to increase 3.6 +/- 1.2-fold within 10 h after mitogen addition. Therefore, the increase in actin synthesis after mitogenic activation seems to be accounted for by accumulation of actin mRNA sequences. Total translatable mRNA and poly(A) sequences also accumulated in parallel with total protein synthesis, suggesting that regulation of actin synthesis was not unique. Two direct studies of mRNA utilization indicated that there is little, if any, translational regulation of actin synthesis. A detailed examination of actin mRNA-containing polysomes and total polysomes revealed no significant change in the average size of polysomes after cell activation. Therefore, given that the rates of polypeptide elongation and termination are constant after mitogen addition (Kay, J.E., Ahern, T., Lindsay V.J., and Sampson, J. (1975) Biochim. Biophys. Acta 378, 241-250), the rate of translational initiation per active mRNA must be unchanged. In addition, no significant amount of unutilized, nonpolysomal actin mRNA was detected in total cell extracts from either unstimulated or activated cells. Together these data suggest that elevated protein synthesis in activated lymphocytes is regulated by mRNA level.

摘要

在有丝分裂原伴刀豆球蛋白A的作用下,牛小淋巴细胞中的蛋白质合成速率在10小时内增加了约3倍,在24小时内增加了约6倍。细胞骨架蛋白肌动蛋白的合成速率与总蛋白质合成速率平行增加,肌动蛋白约占总蛋白质合成的10%。在添加促有丝分裂原后的不同时间,使用来自携带编码牛肌动蛋白片段的重组质粒的cDNA探针测定肌动蛋白mRNA的细胞水平。发现肌动蛋白mRNA序列在3小时内显著增加,在添加促有丝分裂原后10小时内增加了3.6±1.2倍。因此,有丝分裂原激活后肌动蛋白合成的增加似乎是由肌动蛋白mRNA序列的积累引起的。总可翻译mRNA和聚腺苷酸序列也与总蛋白质合成平行积累,这表明肌动蛋白合成的调节并非独特。两项对mRNA利用的直接研究表明,即使有,对肌动蛋白合成的翻译调控也很少。对含有肌动蛋白mRNA的多核糖体和总多核糖体的详细检查显示,细胞激活后多核糖体的平均大小没有显著变化。因此,鉴于添加促有丝分裂原后多肽延伸和终止的速率是恒定的(凯,J.E.,埃亨,T.,林赛V.J.和桑普森,J.(1975年)《生物化学与生物物理学报》378,241 - 250),每个活性mRNA的翻译起始速率必须不变。此外,在未刺激或激活细胞的总细胞提取物中未检测到大量未利用的、非多核糖体的肌动蛋白mRNA。这些数据共同表明,激活淋巴细胞中蛋白质合成的增加是由mRNA水平调节的。

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