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叶绿体核糖核蛋白作为基质中无核糖体mRNA的稳定因子发挥作用。

Chloroplast ribonucleoproteins function as a stabilizing factor of ribosome-free mRNAs in the stroma.

作者信息

Nakamura T, Ohta M, Sugiura M, Sugita M

机构信息

Center for Gene Research, Nagoya University, Nagoya 464-8601, Japan.

出版信息

J Biol Chem. 2001 Jan 5;276(1):147-52. doi: 10.1074/jbc.M008817200.

Abstract

Post-transcriptional RNA processing is an important step in the regulation of chloroplast gene expression, and a number of chloroplast ribonucleoproteins (cpRNPs) are likely to be involved in this process. The major tobacco cpRNPs are composed of five species: cp28, cp29A, cp29B, cp31, and cp33 and these are divided into three groups (I, II, and III). By immunoprecipitation, gel filtration, and Western blot analysis, we demonstrated that these cpRNPs are abundant stromal proteins that exist as complexes with ribosome-free mRNAs. Many ribosome-free psbA mRNAs coprecipitate with cpRNPs, indicating that the majority of stromal psbA mRNAs are associated with cpRNPs. In addition, an in vitro mRNA degradation assay indicated that exogenous psbA mRNA is more rapidly degraded in cpRNP-depleted extracts than in nondepleted extracts. When the depleted extract was reconstituted with recombinant cpRNPs, the psbA mRNA in the extract was protected from degradation to a similar extent as the psbA mRNA in the nondepleted extract. Moreover, restoration of the stabilizing activity varied following addition of individual group-specific cpRNPs alone or in combination. When the five cpRNPs were supplemented in the depleted extract, full activity was restored. We propose that these cpRNPs act as stabilizing factors for nonribosome-bound mRNAs in the stroma.

摘要

转录后RNA加工是叶绿体基因表达调控中的一个重要步骤,许多叶绿体核糖核蛋白(cpRNP)可能参与了这一过程。烟草中的主要cpRNP由五种组成:cp28、cp29A、cp29B、cp31和cp33,它们被分为三组(I、II和III)。通过免疫沉淀、凝胶过滤和蛋白质免疫印迹分析,我们证明这些cpRNP是丰富的基质蛋白,它们以与无核糖体mRNA形成复合物的形式存在。许多无核糖体的psbA mRNA与cpRNP共沉淀,这表明大多数基质中的psbA mRNA与cpRNP相关联。此外,体外mRNA降解试验表明,外源psbA mRNA在cpRNP缺失的提取物中比在未缺失的提取物中降解得更快。当用重组cpRNP对缺失提取物进行重建时,提取物中的psbA mRNA受到的降解保护程度与未缺失提取物中的psbA mRNA相似。此外,单独或组合添加个别组特异性cpRNP后,稳定活性的恢复情况有所不同。当在缺失提取物中补充这五种cpRNP时,可恢复全部活性。我们认为这些cpRNP作为基质中无核糖体结合mRNA的稳定因子发挥作用。

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