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利用三维共聚焦和扫描电子显微镜原位探测拟南芥叶片质体的体积。

Probing the in situ volumes of Arabidopsis leaf plastids using three-dimensional confocal and scanning electron microscopy.

机构信息

School of Biological Sciences, Washington State University, P.O. Box 644236, Pullman, Washington, 99164-4236, USA.

Institute of Plant Biology and Biotechnology, University of Münster, Schlossplatz 7, 48149, Münster, Germany.

出版信息

Plant J. 2024 Jan;117(2):332-341. doi: 10.1111/tpj.16554. Epub 2023 Nov 20.

DOI:10.1111/tpj.16554
PMID:37985241
Abstract

Leaf plastids harbor a plethora of biochemical reactions including photosynthesis, one of the most important metabolic pathways on Earth. Scientists are eager to unveil the physiological processes within the organelle but also their interconnection with the rest of the plant cell. An increasingly important feature of this venture is to use experimental data in the design of metabolic models. A remaining obstacle has been the limited in situ volume information of plastids and other cell organelles. To fill this gap for chloroplasts, we established three microscopy protocols delivering in situ volumes based on: (i) chlorophyll fluorescence emerging from the thylakoid membrane, (ii) a CFP marker embedded in the envelope, and (iii) calculations from serial block-face scanning electron microscopy (SBFSEM). The obtained data were corroborated by comparing wild-type data with two mutant lines affected in the plastid division machinery known to produce small and large mesophyll chloroplasts, respectively. Furthermore, we also determined the volume of the much smaller guard cell plastids. Interestingly, their volume is not governed by the same components of the division machinery which defines mesophyll plastid size. Based on our three approaches, the average volume of a mature Col-0 wild-type mesophyll chloroplasts is 93 μm . Wild-type guard cell plastids are approximately 18 μm . Lastly, our comparative analysis shows that the chlorophyll fluorescence analysis can accurately determine chloroplast volumes, providing an important tool to research groups without access to transgenic marker lines expressing genetically encoded fluorescence proteins or costly SBFSEM equipment.

摘要

叶绿体是一个复杂的细胞器,含有多种生化反应,包括地球上最重要的代谢途径之一光合作用。科学家们渴望揭示细胞器内的生理过程,以及它们与植物细胞其他部分的相互联系。这项研究的一个日益重要的特点是在代谢模型设计中使用实验数据。一个遗留的障碍是叶绿体和其他细胞细胞器的原位体积信息有限。为了填补这一空白,我们建立了三种基于以下三种方法的显微镜方案来提供原位体积信息:(i)来自类囊体膜的叶绿素荧光,(ii)嵌入在包膜中的 CFP 标记,以及(iii)来自连续块面扫描电子显微镜(SBFSEM)的计算。通过将野生型数据与两种分别影响叶绿体分裂机制的突变体系进行比较,验证了所获得的数据。这两种突变体系分别产生小和大的叶肉叶绿体。此外,我们还确定了体积小得多的保卫细胞叶绿体的体积。有趣的是,它们的体积不受分裂机制的相同组件控制,而这些组件决定了叶肉叶绿体的大小。基于我们的三种方法,成熟 Col-0 野生型叶肉叶绿体的平均体积为 93μm。野生型保卫细胞叶绿体的体积约为 18μm。最后,我们的比较分析表明,叶绿素荧光分析可以准确地确定叶绿体的体积,为没有获得表达遗传编码荧光蛋白的转基因标记系或昂贵的 SBFSEM 设备的研究小组提供了一个重要的工具。

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