Messenger RNA enrichment using synthetic oligo(T) click nucleic acids

被引:9
作者
Anderson, Alex J. [1 ]
Culver, Heidi R. [1 ]
Prieto, Tania R. [1 ]
Martinez, Payton J. [1 ]
Sinha, Jasmine [1 ]
Bryant, Stephanie J. [1 ,2 ,3 ]
Bowman, Christopher N. [1 ,2 ,3 ]
机构
[1] Univ Colorado, Dept Chem & Biol Engn, Boulder, CO 80303 USA
[2] Univ Colorado, Mat Sci & Engn Program, Boulder, CO 80303 USA
[3] Univ Colorado, BioFrontiers Inst, Boulder, CO 80303 USA
关键词
HYBRIDIZATION; BIOMARKER; SEQ;
D O I
10.1039/d0cc05815g
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
Enrichment of mRNA is a key step in a number of molecular biology techniques, particularly in the rapidly growing field of transcriptomics. Currently, mRNA is isolated using oligo(thymine) DNA (oligo(dT)) immobilized on solid supports, which binds to the poly(A) tail of mRNA to pull the mRNA out of solution through the use of magnets or centrifugal filters. Here, a simple method to isolate mRNA by complexing it with synthetic click nucleic acids (CNAs) is described. Oligo(T) CNA bound efficiently to mRNA, and because of the insolubility of CNA in water, >90% of mRNA was readily removed from solution using this method. Simple washing, buffer exchange, and heating steps enabled mRNA's enrichment from total RNA, with a yield of 3.1 +/- 1.5% of the input total RNA by mass, comparable to the yield from commercially available mRNA enrichment beads. Further, the integrity and activity of mRNA after CNA-facilitated pulldown and release was evaluated through two assays. In vitro translation of EGFP mRNA confirmed the translatability of mRNA into functional protein and RT-qPCR was used to amplify enriched mRNA from total RNA extracts and compare gene expression to results obtained using commercially available products.
引用
收藏
页码:13987 / 13990
页数:4
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