Literature DB >> 27911841

High-performance multiplexed fluorescence in situ hybridization in culture and tissue with matrix imprinting and clearing.

Jeffrey R Moffitt1,2, Junjie Hao1,2, Dhananjay Bambah-Mukku1,3, Tian Lu1,2, Catherine Dulac1,3, Xiaowei Zhuang4,2,5.   

Abstract

Highly multiplexed single-molecule FISH has emerged as a promising approach to spatially resolved single-cell transcriptomics because of its ability to directly image and profile numerous RNA species in their native cellular context. However, background-from off-target binding of FISH probes and cellular autofluorescence-can become limiting in a number of important applications, such as increasing the degree of multiplexing, imaging shorter RNAs, and imaging tissue samples. Here, we developed a sample clearing approach for FISH measurements. We identified off-target binding of FISH probes to cellular components other than RNA, such as proteins, as a major source of background. To remove this source of background, we embedded samples in polyacrylamide, anchored RNAs to this polyacrylamide matrix, and cleared cellular proteins and lipids, which are also sources of autofluorescence. To demonstrate the efficacy of this approach, we measured the copy number of 130 RNA species in cleared samples using multiplexed error-robust FISH (MERFISH). We observed a reduction both in the background because of off-target probe binding and in the cellular autofluorescence without detectable loss in RNA. This process led to an improved detection efficiency and detection limit of MERFISH, and an increased measurement throughput via extension of MERFISH into four color channels. We further demonstrated MERFISH measurements of complex tissue samples from the mouse brain using this matrix-imprinting and -clearing approach. We envision that this method will improve the performance of a wide range of in situ hybridization-based techniques in both cell culture and tissues.

Entities:  

Keywords:  brain; fluorescence in situ hybridization; multiplexed imaging; single-cell transcriptomics; tissue clearing

Mesh:

Substances:

Year:  2016        PMID: 27911841      PMCID: PMC5167177          DOI: 10.1073/pnas.1617699113

Source DB:  PubMed          Journal:  Proc Natl Acad Sci U S A        ISSN: 0027-8424            Impact factor:   11.205


  46 in total

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Review 7.  In the right place at the right time: visualizing and understanding mRNA localization.

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