大肠杆菌色氨酸酶的无细胞合成。使用从诱导细胞中分离的核糖核酸，并比较采用核糖体的系统与采用核糖体和外源核糖核酸的系统所产生的产物。

Cell-free synthesis of tryptophanase from Escherichia coli. Use of ribonucleic acid isolated from induced cells and a comparison of the product from a system employing ribosomes with that from one employing ribosomes and exogenous ribonucleic acid.

作者信息

Parish J H, Khairul Bashar S A, Brown N L, Brown M

出版信息

Biochem J. 1971 Nov;125(2):643-53. doi: 10.1042/bj1250643.

DOI:10.1042/bj1250643

PMID:4947396

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC1178102/

Abstract

Polyribosomes and RNA were isolated from cultures in which tryptophanase (EC 4.2.1.-) was induced. The polyribosomes were incubated under conditions of protein synthesis, in the presence of a radioactive amino acid and a post-ribosomal supernatant fraction obtained from repressed cells. The RNA preparations were incubated under conditions of protein synthesis in the presence of a radioactive amino acid and a supernatant fraction containing ribosomes from repressed cells. 2. The system was characterized and the synthesis of a radioactive protein with the same chromatographic properties as tryptophanase was demonstrated. This synthesis was shown to be time-dependent and required the presence of RNA from induced cultures, ribosomes and an energy supply; it was inhibited by chloramphenicol. 3. The maximum activity for the synthesis of this protein was found to be associated with 23S rRNA isolated from sucrose gradients. 4. The N-terminal amino acid of tryptophanase was labelled in the protein synthesized in this system but not in the protein synthesized by polyribosomes (without added RNA). Conversely, the C-terminal amino acid of tryptophanase was labelled in the polyribosome system but not in the RNA-containing system. 5. Tryptic digests of protein labelled in vitro were compared with those of tryptophanase. No labelled tryptic peptides were identified other than tryptophanase tryptic peptides. An analysis of the results implied that in the polyribosome system almost the complete tryptophanase subunit chain was labelled but that in the RNA-containing system these chains were incompletely synthesized. 6. Sucrose-gradient analysis of protein synthesized in the RNA-containing system suggested that it cannot be converted into structures with the same sedimentation properties as native tryptophanase. 7. The significance of these results for the assay of tryptophanase mRNA and for an understanding of the control of the translation of this mRNA in vivo is discussed.

摘要

从诱导产生色氨酸酶（EC 4.2.1.-）的培养物中分离出多核糖体和RNA。将多核糖体在蛋白质合成条件下，于放射性氨基酸和从阻遏细胞获得的核糖体后上清液组分存在的情况下进行温育。RNA制剂在蛋白质合成条件下，于放射性氨基酸和含有来自阻遏细胞核糖体的上清液组分存在的情况下进行温育。2. 对该系统进行了表征，并证明合成了具有与色氨酸酶相同色谱性质的放射性蛋白质。这种合成显示出时间依赖性，并且需要来自诱导培养物的RNA、核糖体和能量供应；它受到氯霉素的抑制。3. 发现合成这种蛋白质的最大活性与从蔗糖梯度中分离出的23S rRNA相关。4. 在该系统中合成的蛋白质中色氨酸酶的N末端氨基酸被标记，但在多核糖体（未添加RNA）合成的蛋白质中未被标记。相反，色氨酸酶的C末端氨基酸在多核糖体系统中被标记，但在含RNA的系统中未被标记。5. 将体外标记的蛋白质的胰蛋白酶消化产物与色氨酸酶的消化产物进行比较。除了色氨酸酶的胰蛋白酶肽段外，未鉴定出其他标记的胰蛋白酶肽段。对结果的分析表明，在多核糖体系统中几乎完整的色氨酸酶亚基链被标记，但在含RNA的系统中这些链未完全合成。6. 对含RNA系统中合成的蛋白质进行蔗糖梯度分析表明，它不能转化为具有与天然色氨酸酶相同沉降性质的结构。7. 讨论了这些结果对于色氨酸酶mRNA测定以及理解该mRNA在体内翻译控制的意义。