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体内叶绿素荧光筛选可分离出一个 Chlamydomonas 突变体,该突变体缺乏参与线粒体复合物 I 组装的组装因子 NDUFAF3。

In vivo chlorophyll fluorescence screening allows the isolation of a Chlamydomonas mutant defective for NDUFAF3, an assembly factor involved in mitochondrial complex I assembly.

机构信息

InBioS - Genetics and Physiology of Microalgae, Chemin de la vallée, 4, 4000 Liège, University of Liège, Belgium.

PhytoSYSTEMS, Chemin de la vallée, 4, 4000 Liège, University of Liège, Belgium.

出版信息

Plant J. 2017 Nov;92(4):584-595. doi: 10.1111/tpj.13677. Epub 2017 Sep 28.

DOI:10.1111/tpj.13677
PMID:28857403
Abstract

The qualitative screening method used to select complex I mutants in the microalga Chlamydomonas, based on reduced growth under heterotrophic conditions, is not suitable for high-throughput screening. In order to develop a fast screening method based on measurements of chlorophyll fluorescence, we first demonstrated that complex I mutants displayed decreased photosystem II efficiency in the genetic background of a photosynthetic mutation leading to reduced formation of the electrochemical proton gradient in the chloroplast (pgrl1 mutation). In contrast, single mutants (complex I and pgrl1 mutants) could not be distinguished from the wild type by their photosystem II efficiency under the conditions tested. We next performed insertional mutagenesis on the pgrl1 mutant. Out of about 3000 hygromycin-resistant insertional transformants, 46 had decreased photosystem II efficiency and three were complex I mutants. One of the mutants was tagged and whole genome sequencing identified the resistance cassette in NDUFAF3, a homolog of the human NDUFAF3 gene, encoding for an assembly factor involved in complex I assembly. Complemented strains showed restored complex I activity and assembly. Overall, we describe here a screening method which is fast and particularly suited for the identification of Chlamydomonas complex I mutants.

摘要

用于从衣藻中筛选复杂 I 突变体的定性筛选方法基于异养条件下生长减少,但不适合高通量筛选。为了开发基于叶绿素荧光测量的快速筛选方法,我们首先证明在导致叶绿体中电化学质子梯度形成减少的光合突变(pgrl1 突变)的遗传背景下,复杂 I 突变体显示出光合作用 II 效率降低。相比之下,在测试条件下,单突变体(复杂 I 和 pgrl1 突变体)不能与其光合作用 II 效率从野生型中区分开来。我们接下来在 pgrl1 突变体上进行插入诱变。在大约 3000 个潮霉素抗性插入转化体中,有 46 个表现出光合作用 II 效率降低,其中 3 个是复杂 I 突变体。其中一个突变体被标记,全基因组测序确定了抗性盒在 NDUFAF3 中的位置,NDUFAF3 是人 NDUFAF3 基因的同源物,编码参与复杂 I 组装的组装因子。互补株系显示出恢复的复杂 I 活性和组装。总的来说,我们在这里描述了一种快速筛选方法,特别适合鉴定衣藻复杂 I 突变体。

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