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Ultra-high throughput single-cell analysis of proteins and RNAs by split-pool synthesis

Articolo
Data di Pubblicazione:
2020
Abstract:
Abstract Single-cell omics provide insight into cellular heterogeneity and function. Recent technological advances have accelerated single-cell analyses, but workflows remain expensive and complex. We present a method enabling simultaneous, ultra-high throughput single-cell barcoding of millions of cells for targeted analysis of proteins and RNAs. Quantum barcoding (QBC) avoids isolation of single cells by building cell-specific oligo barcodes dynamically within each cell. With minimal instrumentation (four 96-well plates and a multichannel pipette), cell-specific codes are added to each tagged molecule within cells through sequential rounds of classical split-pool synthesis. Here we show the utility of this technology in mouse and human model systems for as many as 50 antibodies to targeted proteins and, separately, >70 targeted RNA regions. We demonstrate that this method can be applied to multi-modal protein and RNA analyses. It can be scaled by expansion of the split-pool process and effectively renders sequencing instruments as versatile multi-parameter flow cytometers.
Tipologia CRIS:
1.1 Articolo in rivista
Elenco autori:
O’Huallachain, Maeve; Bava, F; Shen, Mary; Dallett, Carolina; Paladugu, Sri; Samusik, Nikolay; Yu, Simon; Hussein, Razika; Hillman Grantland, R.; Higgins, Samuel; Lou, Melanie; Trejo, Angelica; Qin, Laura; Tai Yu, Chuan; Kinoshita Shigemi, M.; Jager, Astraea; Lashkari, Deval; Goltsev, Yury; Ozturk, Sedide; Nolan Garry, P.
Link alla scheda completa:
https://iris.unilink.it/handle/20.500.14085/28641
Pubblicato in:
COMMUNICATIONS BIOLOGY
Journal
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URL

http://www.nature.com/articles/s42003-020-0896-2
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