Breaking barriers: improving time and space resolution of arbuscular mycorrhizal symbiosis with single-cell sequencing approaches.

IF 5.7 2区 生物学 Q1 BIOLOGY
Sofía Cristina Somoza, Paola Bonfante, Marco Giovannetti
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Abstract

The cell and molecular bases of arbuscular mycorrhizal (AM) symbiosis, a crucial plant-fungal interaction for nutrient acquisition, have been extensively investigated by coupling traditional RNA sequencing techniques of roots sampled in bulk, with methods to capture subsets of cells such as laser microdissection. These approaches have revealed central regulators of this complex relationship, yet the requisite level of detail to effectively untangle the intricacies of temporal and spatial development remains elusive.The recent adoption of single-cell RNA sequencing (scRNA-seq) techniques in plant research is revolutionizing our ability to dissect the intricate transcriptional profiles of plant-microbe interactions, offering unparalleled insights into the diversity and dynamics of individual cells during symbiosis. The isolation of plant cells is particularly challenging due to the presence of cell walls, leading plant researchers to widely adopt nuclei isolation methods. Despite the increased resolution that single-cell analyses offer, it also comes at the cost of spatial perspective, hence, it is necessary the integration of these approaches with spatial transcriptomics to obtain a comprehensive overview.To date, few single-cell studies on plant-microbe interactions have been published, most of which provide high-resolution cell atlases that will become crucial for fully deciphering symbiotic interactions and addressing future questions. In AM symbiosis research, key processes such as the mutual recognition of partners during arbuscule development within cortical cells, or arbuscule senescence and degeneration, remain poorly understood, and these advancements are expected to shed light on these processes and contribute to a deeper understanding of this plant-fungal interaction.

打破障碍:利用单细胞测序方法提高假根菌根共生的时空分辨率。
根瘤菌共生是植物与真菌之间获取养分的重要互动关系,通过对根系进行大量取样的传统 RNA 测序技术与激光显微切割等捕获细胞子集的方法相结合,对根瘤菌共生的细胞和分子基础进行了广泛研究。最近在植物研究中采用的单细胞 RNA 测序(scRNA-seq)技术正在彻底改变我们剖析植物与微生物相互作用的复杂转录图谱的能力,为我们提供了对共生过程中单个细胞的多样性和动态的无与伦比的洞察力。由于细胞壁的存在,植物细胞的分离尤其具有挑战性,因此植物研究人员广泛采用细胞核分离方法。尽管单细胞分析提高了分辨率,但也付出了空间视角的代价,因此有必要将这些方法与空间转录组学结合起来,以获得全面的概述。迄今为止,有关植物与微生物相互作用的单细胞研究很少发表,其中大多数都提供了高分辨率的细胞图谱,这将成为全面解密共生相互作用和解决未来问题的关键。在AM共生研究中,诸如在皮层细胞内轴突发育过程中伙伴间的相互识别或轴突衰老和退化等关键过程仍然鲜为人知,这些进展有望揭示这些过程,并有助于加深对这种植物-真菌相互作用的理解。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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来源期刊
Biology Direct
Biology Direct 生物-生物学
CiteScore
6.40
自引率
10.90%
发文量
32
审稿时长
7 months
期刊介绍: Biology Direct serves the life science research community as an open access, peer-reviewed online journal, providing authors and readers with an alternative to the traditional model of peer review. Biology Direct considers original research articles, hypotheses, comments, discovery notes and reviews in subject areas currently identified as those most conducive to the open review approach, primarily those with a significant non-experimental component.
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