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完整制备淋巴腺以全面分析幼虫造血过程。

Intact Preparation of the Lymph Gland for a Comprehensive Analysis of Larval Hematopoiesis.

作者信息

Rodrigues Diana, VijayRaghavan K, Waltzer Lucas, Inamdar Maneesha S

机构信息

Jawaharlal Nehru Centre for Advanced Scientific Research, Bangalore, India.

National Centre for Biological Sciences, Tata Institute of Fundamental Research, Bangalore, India.

出版信息

Bio Protoc. 2021 Nov 5;11(21):e4204. doi: 10.21769/BioProtoc.4204.

Abstract

Blood cells have a limited lifespan and are replenished by a small number of hematopoietic stem and progenitor cells (HSPCs). Adult vertebrate hematopoiesis occurs in the bone marrow, liver, and spleen, rendering a comprehensive analysis of the entire HSPC pool nearly impossible. The blood system is well studied and has developmental, molecular, and functional parallels with that of vertebrates. Unlike vertebrates, post-embryonic hematopoiesis in is essentially restricted to the larval lymph gland (LG), a multi-lobed organ that flanks the dorsal vessel. Because the anterior-most or primary lobes of the LG are easy to dissect out, their cellular and molecular characteristics have been studied in considerable detail. The 2-3 pairs of posterior lobes are more delicate and fragile and have largely been ignored. However, posterior lobes harbor a significant blood progenitor pool, and several hematopoietic mutants show differences in phenotype between the anterior and posterior lobes. Hence, a comprehensive analysis of the LG is important for a thorough understanding of hematopoiesis. Most studies focus on isolating the primary lobes by methods that generally dislodge and damage other lobes. To obtain preparations of the whole LG, including intact posterior lobes, here we provide a detailed protocol for larval fillet dissection. This allows accessing and analyzing complete LG lobes, along with dorsal vessel and pericardial cells. We demonstrate that tissue architecture and integrity is maintained and provide methods for quantitative analysis. This protocol can be used to quickly and effectively isolate complete LGs from first instar larval to pupal stages and can be implemented with ease.

摘要

血细胞寿命有限,由少量造血干细胞和祖细胞(HSPCs)补充。成年脊椎动物的造血过程发生在骨髓、肝脏和脾脏中,因此几乎不可能对整个HSPC库进行全面分析。血液系统已得到充分研究,在发育、分子和功能方面与脊椎动物的血液系统有相似之处。与脊椎动物不同,果蝇胚胎后的造血过程基本上局限于幼虫淋巴腺(LG),这是一个位于背血管两侧的多叶器官。由于LG最前端或主要叶很容易解剖出来,因此对其细胞和分子特征进行了相当详细的研究。2-3对后叶更为精细和脆弱,在很大程度上被忽视了。然而,后叶含有大量的血液祖细胞库,一些造血突变体在前叶和后叶之间表现出表型差异。因此,对LG进行全面分析对于深入了解果蝇造血过程很重要。大多数研究集中于通过通常会使其他叶移位和受损的方法分离主要叶。为了获得包括完整后叶在内的整个LG的标本,我们在此提供了一份详细的幼虫去头解剖方案。这使得能够获取和分析完整的LG叶,以及背血管和心包细胞。我们证明了组织结构和完整性得以维持,并提供了定量分析方法。该方案可用于从一龄幼虫到蛹期快速有效地分离完整的LG,且易于实施。

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