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激光显微切割RNA测序的实验设计:来自玉米叶片发育分析的经验教训

Experimental Design for Laser Microdissection RNA-Seq: Lessons from an Analysis of Maize Leaf Development.

作者信息

Johnston Robyn M, Sylvester Anne W, Scanlon Michael J

机构信息

Plant Biology Section, School of Integrative Plant Science, Cornell University.

Department of Developmental Genetics, University of Wyoming.

出版信息

J Vis Exp. 2017 Mar 5(121):55004. doi: 10.3791/55004.

Abstract

Genes with important roles in development frequently have spatially and/or temporally restricted expression patterns. Often these gene transcripts are not detected or are not identified as differentially expressed (DE) in transcriptomic analyses of whole plant organs. Laser Microdissection RNA-Seq (LM RNA-Seq) is a powerful tool to identify genes that are DE in specific developmental domains. However, the choice of cellular domains to microdissect and compare, and the accuracy of the microdissections are crucial to the success of the experiments. Here, two examples illustrate design considerations for transcriptomics experiments; a LM RNA-seq analysis to identify genes that are DE along the maize leaf proximal-distal axis, and a second experiment to identify genes that are DE in liguleless1-R (lg1-R) mutants compared to wild-type. Key elements that contributed to the success of these experiments were detailed histological and in situ hybridization analyses of the region to be analyzed, selection of leaf primordia at equivalent developmental stages, the use of morphological landmarks to select regions for microdissection, and microdissection of precisely measured domains. This paper provides a detailed protocol for the analysis of developmental domains by LM RNA-Seq. The data presented here illustrate how the region selected for microdissection will affect the results obtained.

摘要

在发育过程中起重要作用的基因通常具有空间和/或时间上受限的表达模式。在对整个植物器官进行转录组分析时,这些基因转录本往往未被检测到或未被鉴定为差异表达(DE)。激光显微切割RNA测序(LM RNA-Seq)是一种强大的工具,可用于鉴定在特定发育区域中差异表达的基因。然而,选择用于显微切割和比较的细胞区域以及显微切割的准确性对于实验的成功至关重要。在这里,两个例子说明了转录组学实验的设计考虑因素:一个用于鉴定沿玉米叶片近-远轴差异表达基因的LM RNA-seq分析,以及另一个用于鉴定与野生型相比在liguleless1-R(lg1-R)突变体中差异表达基因的实验。促成这些实验成功的关键因素包括对要分析的区域进行详细的组织学和原位杂交分析、选择处于等效发育阶段的叶原基、使用形态学标记来选择显微切割区域以及对精确测量的区域进行显微切割。本文提供了一份通过LM RNA-Seq分析发育区域的详细方案。此处呈现的数据说明了选择用于显微切割的区域将如何影响所获得的结果。

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本文引用的文献

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