Mime-seq 2.0: a method to sequence microRNAs from specific mouse cell types

Author:

Mandlbauer ArianeORCID,Sun Qiong,Popitsch NikoORCID,Schwickert TanjaORCID,Spanova Miroslava,Wang JingkuiORCID,Ameres StefanORCID,Busslinger MeinradORCID,Cochella LuisaORCID

Abstract

AbstractMany microRNAs (miRNAs) are expressed with high spatiotemporal specificity during organismal development, with some being limited to rare cell types, often embedded in complex tissues. Yet most miRNA profiling efforts remain at the tissue and organ levels. To overcome challenges in accessing the microRNomes from tissue-embedded cells, we had previously developed mime-seq (miRNome bymethylation dependent sequencing), a technique in which cell-specific miRNA methylation inC. elegansandDrosophilaenabled chemo-selective sequencing without the need for cell sorting or biochemical purification. Here, we present mime-seq 2.0 for profiling miRNAs from specific mouse cell types. We engineered a chimeric RNA methyltransferase that is tethered to Argonaute and efficiently methylates miRNAs at their 3’-terminal 2’OH in mouse and human cell lines. We also generated a transgenic mouse for conditional expression of this methyltransferase, which can be used to direct methylation of miRNAs in a cell-type of choice. We validated the use of this mouse by profiling miRNAs from B cells and bone marrow plasma cells.

Publisher

Cold Spring Harbor Laboratory

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