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Merck

iTAG-RNA Isolates Cell-Specific Transcriptional Responses to Environmental Stimuli and Identifies an RNA-Based Endocrine Axis.

Cell reports (2020-03-05)
Jonatan Darr, Archana Tomar, Maximilian Lassi, Raffaele Gerlini, Lucia Berti, Annette Hering, Fabienne Scheid, Martin Hrabฤ› de Angelis, Michael Witting, Raffaele Teperino
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Biofluids contain various circulating cell-free RNAs (ccfRNAs). The composition of these ccfRNAs variesย among biofluids. They constitute tantalizing biomarker candidates for several pathologies and have been demonstrated to be mediators of cellular communication. Little is known about their function in physiological and developmental settings, and most works are limited to inย vitro studies. Here, we develop iTAG-RNA, a method for the unbiased tagging of RNA transcripts in mice inย vivo. We use iTAG-RNA to isolate hepatocytes and kidney proximal epithelial cell-specific transcriptional responses to a dietary challenge without interfering with the tissue architecture and to identify multiple hepatocyte-secreted ccfRNAs in plasma. We also identify specific transfer of liver-derived ccfRNAs to adipose tissue and skeletal muscle, where they likely constitute a buffering system to maintain lipid homeostasis under acute high-fat-diet feeding. Our findings directly demonstrate inย vivo transfer of RNAs between tissues and highlight its implications for endocrine signaling and homeostasis.

MATERIALS
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5-Ethynyl uridine, ≥95%
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Sodium chloride solution, 0.9% in water, BioXtra, suitable for cell culture
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Formalin solution, neutral buffered, 10%, histological tissue fixative
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Cytidine, BioReagent, suitable for cell culture, powder, ≥99%
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Uridine, ≥99%
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Benzonaseยฎ Nuclease, ultrapure, โ‰ฅ250 units/ฮผL, โ‰ฅ99% (SDS-PAGE), recombinant, expressed in E. coli, buffered aqueous glycerol solution, ultrapure grade
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Azamulin, ≥98% (HPLC)
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SIGMAFASTโ„ข Protease Inhibitor Tablets, For General Use
Millipore
Immobilonยฎ-PSQ PVDF Membrane, 1 roll, 27 cm x 3.75 m, 0.2 ยตm pore size, Hydrophobic PVDF Transfer Membrane for western blotting.
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Phosphodiesterase I from Crotalus adamanteus venom, vial of โ‰ฅ100 units, Purified
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Phosphatase, Alkaline from bovine intestinal mucosa, ≥2,000 DEA units/mg protein
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Adenosine, ≥99%
Supelco
Bradford Reagent, for 0.1-1.4 mg/ml protein
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Guanosine, ≥98%