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优化的新鲜和冷冻固体肿瘤标本的核分离用于多组学测序。

Optimized Nuclei Isolation from Fresh and Frozen Solid Tumor Specimens for Multiome Sequencing.

机构信息

Hagey Laboratory for Pediatric Regenerative Medicine, Department of Surgery, Stanford University.

Hagey Laboratory for Pediatric Regenerative Medicine, Department of Surgery, Stanford University;

出版信息

J Vis Exp. 2023 Oct 13(200). doi: 10.3791/65831.

Abstract

Multiome sequencing, which provides same-cell/paired single-cell RNA- and the assay for transposase-accessible chromatin with sequencing (ATAC-sequencing) data, represents a breakthrough in our ability to discern tumor cell heterogeneity-a primary focus of translational cancer research at this time. However, the quality of sequencing data acquired using this advanced modality is highly dependent on the quality of the input material. Digestion conditions need to be optimized to maximize cell yield without sacrificing quality. This is particularly challenging in the context of solid tumors with dense desmoplastic matrices that must be gently broken down for cell release. Freshly isolated cells from solid tumor tissue are more fragile than those isolated from cell lines. Additionally, as the cell types isolated are heterogeneous, conditions should be selected to support the total cell population. Finally, nuclear isolation conditions must be optimized based on these qualities in terms of lysis times and reagent types/ratios. In this article, we describe our experience with nuclear isolation for the 10x Genomics multiome sequencing platform from solid tumor specimens. We provide recommendations for tissue digestion, storage of single-cell suspensions (if desired), and nuclear isolation and assessment.

摘要

多组学测序,提供单细胞/配对单细胞 RNA 和转座酶可及染色质的测定(ATAC-seq)数据,代表着我们能够识别肿瘤细胞异质性的能力的突破——这是当前转化癌症研究的主要焦点。然而,使用这种先进模式获得的测序数据的质量高度依赖于输入材料的质量。需要优化消化条件以最大限度地提高细胞产量,同时不牺牲质量。对于具有密集纤维基质的实体瘤,这尤其具有挑战性,必须轻柔地破坏纤维基质以释放细胞。从实体瘤组织中分离的新鲜细胞比从细胞系中分离的细胞更脆弱。此外,由于分离的细胞类型具有异质性,应选择条件来支持总细胞群体。最后,必须根据裂解时间和试剂类型/比例等因素优化核分离条件。本文描述了我们在固体肿瘤标本上使用 10x Genomics 多组学测序平台进行核分离的经验。我们提供了有关组织消化、单细胞悬液(如果需要)的储存以及核分离和评估的建议。

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