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从PC12细胞制备无细胞翻译系统。

Preparation of a cell-free translation system from PC12 cell.

作者信息

Shibutani M, Kim E, Lazarovici P, Oshima M, Guroff G

机构信息

Section of Growth Factors, National Institute of Child Health and Human Development, National Institutes of Health, Bethesda, Maryland 20892, USA.

出版信息

Neurochem Res. 1996 Jul;21(7):801-7. doi: 10.1007/BF02532303.

Abstract

The postmitochondrial fraction (S10) contains the cellular components essential for translation, and a high-salt wash (HSW) of the ribosomes is enriched in eukaryotic initiation factors. This report describes the preparation of a cell-free translation system utilizing an S10 extract from PC12 cells. The products synthesized from either firefly luciferase mRNA or PC12 cell poly(A) RNAs in the PC12-S10 extract were increased by the addition of the HSW from PC12 cells. Increases in the translation of luciferase mRNA by the addition of PC12-HSW were dose-dependent and also dependent on the time of incubation. The translation of human epidermal growth factor receptor (hEGFR) mRNA could also be detected in the PC12-S10 extract translation system by immuno-precipitation. N-linked glycosylation of the translation products also was observed. The efficiency of translation was altered by the addition of Mg2- or K+, and optimization of the concentrations of these ions was necessary for each mRNA. The translation system made from PC12 cells, then, is capable of the synthesis of proteins of relatively high molecular weight and should be useful for analyzing mechanisms of translational control during proliferation and differentiation of cells from a neuronal lineage.

摘要

线粒体后组分(S10)包含翻译所必需的细胞成分,核糖体的高盐洗涤物(HSW)富含真核生物起始因子。本报告描述了利用PC12细胞的S10提取物制备无细胞翻译系统的方法。在PC12 - S10提取物中,加入PC12细胞的HSW可增加由萤火虫荧光素酶mRNA或PC12细胞多聚腺苷酸RNA合成的产物。加入PC12 - HSW后荧光素酶mRNA翻译的增加呈剂量依赖性,也取决于孵育时间。通过免疫沉淀也可在PC12 - S10提取物翻译系统中检测到人表皮生长因子受体(hEGFR)mRNA的翻译。还观察到翻译产物的N - 连接糖基化。加入Mg2 +或K +会改变翻译效率,每种mRNA都需要优化这些离子的浓度。因此,由PC12细胞制成的翻译系统能够合成相对高分子量的蛋白质,并且应该有助于分析神经谱系细胞增殖和分化过程中的翻译控制机制。

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