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CITRIC:使用新型温度敏感转移 RNA 在衣藻叶绿体中进行冷诱导的翻译通读。

CITRIC: cold-inducible translational readthrough in the chloroplast of Chlamydomonas reinhardtii using a novel temperature-sensitive transfer RNA.

机构信息

Algal Research Group, Institute of Structural and Molecular Biology, University College London, Gower Street, London, WC1E 6BT, UK.

Department of Medicine, Sir Alexander Fleming Building, Imperial College London, South Kensington Campus, London, SW7 2AZ, UK.

出版信息

Microb Cell Fact. 2018 Nov 24;17(1):186. doi: 10.1186/s12934-018-1033-5.

Abstract

BACKGROUND

The chloroplast of eukaryotic microalgae such as Chlamydomonas reinhardtii is a potential platform for metabolic engineering and the production of recombinant proteins. In industrial biotechnology, inducible expression is often used so that the translation or function of the heterologous protein does not interfere with biomass accumulation during the growth stage. However, the existing systems used in bacterial or fungal platforms do not transfer well to the microalgal chloroplast. We sought to develop a simple inducible expression system for the microalgal chloroplast, exploiting an unused stop codon (TGA) in the plastid genome. We have previously shown that this codon can be translated as tryptophan when we introduce into the chloroplast genome a trnW gene encoding a plastidial transfer RNA with a modified anticodon sequence, UCA.

RESULTS

A mutated version of our trnW gene was developed that encodes a temperature-sensitive variant of the tRNA. This allows transgenes that have been modified to contain one or more internal TGA codons to be translated differentially according to the culture temperature, with a gradient of recombinant protein accumulation from 35 °C (low/off) to 15 °C (high). We have named this the CITRIC system, an acronym for cold-inducible translational readthrough in chloroplasts. The exact induction behaviour can be tailored by altering the number of TGA codons within the transgene.

CONCLUSIONS

CITRIC adds to the suite of genetic engineering tools available for the microalgal chloroplast, allowing a greater degree of control over the timing of heterologous protein expression. It could also be used as a heat-repressible system for studying the function of essential native genes in the chloroplast. The genetic components of CITRIC are entirely plastid-based, so no engineering of the nuclear genome is required.

摘要

背景

真核微藻(如莱茵衣藻)的叶绿体是代谢工程和重组蛋白生产的潜在平台。在工业生物技术中,常使用诱导表达,以使异源蛋白的翻译或功能不会在生长阶段干扰生物量积累。然而,在细菌或真菌平台中使用的现有系统并不能很好地转移到微藻叶绿体。我们试图开发一种简单的微藻叶绿体诱导表达系统,利用质体基因组中一个未使用的终止密码子(TGA)。我们之前已经表明,当我们将一个编码带有修饰的反密码子序列 UCA 的质体转移 RNA 的 trnW 基因引入质体基因组时,这个密码子可以被翻译成色氨酸。

结果

开发了一种突变版本的 trnW 基因,该基因编码一种温度敏感型 tRNA。这使得经过修饰的转基因可以根据培养温度以不同的方式翻译,带有一个或多个内部 TGA 密码子的转基因在 35°C(低/关)到 15°C(高)的温度梯度下积累不同水平的重组蛋白。我们将其命名为 CITRIC 系统,是叶绿体冷诱导翻译通读的缩写。通过改变转基因内 TGA 密码子的数量,可以精确调整诱导行为。

结论

CITRIC 增加了可用于微藻叶绿体的遗传工程工具套件,允许在异源蛋白表达的时间上有更大的控制程度。它也可以用作研究叶绿体中必需的天然基因功能的热抑制系统。CITRIC 的遗传元件完全基于质体,因此不需要核基因组的工程改造。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/9348/6260665/2d684aea1d27/12934_2018_1033_Fig1_HTML.jpg

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