A new cell culture resource for investigations of reptilian gene function.

IF 3.7 2区生物学 Q1 DEVELOPMENTAL BIOLOGY

Development Pub Date : 2024-11-15 Epub Date: 2024-11-22 DOI:10.1242/dev.204275

Sukhada P Samudra, Sungdae Park, Elizabeth A Esser, Tryggvi P McDonald, Arianna M Borges, Jonathan Eggenschwiler, Douglas B Menke

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引用次数: 0

Abstract

The establishment of CRISPR/Cas9 gene editing in Anolis sagrei has positioned this species as a powerful model for studies of reptilian gene function. To enhance this model, we developed an immortalized lizard fibroblast cell line (ASEC-1) for the exploration of reptilian gene function in cellular processes. We demonstrate the use of this cell line by scrutinizing the role of primary cilia in lizard Hedgehog (Hh) signaling. Using CRISPR/Cas9 mutagenesis, we disrupted the ift88 gene, which is required for ciliogenesis in diverse organisms. We determined that loss of itf88 from lizard cells leads to an absence of primary cilia, a partial derepression of gli1 transcription, and an inability of the cells to respond to the Smoothened agonist, SAG. Through a cross-species analysis of SAG-induced transcriptional responses in cultured limb bud cells, we further determined that ∼46% of genes induced as a response to Hh pathway activation in A. sagrei are also SAG responsive in Mus musculus limb bud cells. Our results highlight conserved and diverged aspects of Hh signaling in anoles and establish a new resource for investigations of reptilian gene function.

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研究爬行动物基因功能的新细胞培养资源。

CRISPR/Cas9基因编辑技术在巨蜥身上的应用，使该物种成为研究爬行动物基因功能的强大模型。为了加强这一模型，我们开发了一种永生化蜥蜴成纤维细胞系（ASEC-1），用于探索爬行动物基因在细胞过程中的功能。我们通过研究初级纤毛在蜥蜴刺猬（Hh）信号传导中的作用，证明了这一细胞系的用途。我们使用 CRISPR/Cas9 诱变技术破坏了 ift88 基因，该基因是多种生物纤毛生成所必需的。我们发现，蜥蜴细胞中itf88基因的缺失会导致初级纤毛的缺失、gli1转录的部分抑制以及细胞无法对Smoothened激动剂SAG做出反应。通过对培养的肢芽细胞中SAG诱导的转录反应进行跨物种分析，我们进一步确定了在A. sagrei中作为对Hh通路激活的反应而诱导的基因中，有46%的基因在麝香草肢芽细胞中也对SAG有反应。我们的研究结果突显了蝾螈Hh信号转导的保守性和差异性，为研究爬行动物的基因功能提供了新的资源。

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来源期刊

Development 生物-发育生物学

CiteScore

6.70

自引率

4.30%

发文量

433

审稿时长

3 months

期刊介绍： Development’s scope covers all aspects of plant and animal development, including stem cell biology and regeneration. The single most important criterion for acceptance in Development is scientific excellence. Research papers (articles and reports) should therefore pose and test a significant hypothesis or address a significant question, and should provide novel perspectives that advance our understanding of development. We also encourage submission of papers that use computational methods or mathematical models to obtain significant new insights into developmental biology topics. Manuscripts that are descriptive in nature will be considered only when they lay important groundwork for a field and/or provide novel resources for understanding developmental processes of broad interest to the community. Development includes a Techniques and Resources section for the publication of new methods, datasets, and other types of resources. Papers describing new techniques should include a proof-of-principle demonstration that the technique is valuable to the developmental biology community; they need not include in-depth follow-up analysis. The technique must be described in sufficient detail to be easily replicated by other investigators. Development will also consider protocol-type papers of exceptional interest to the community. We welcome submission of Resource papers, for example those reporting new databases, systems-level datasets, or genetic resources of major value to the developmental biology community. For all papers, the data or resource described must be made available to the community with minimal restrictions upon publication. To aid navigability, Development has dedicated sections of the journal to stem cells & regeneration and to human development. The criteria for acceptance into these sections is identical to those outlined above. Authors and editors are encouraged to nominate appropriate manuscripts for inclusion in one of these sections.