Demodifying RNA for Transcriptomic Analyses of Archival Formalin-Fixed Paraffin-Embedded Samples

被引:14
|
作者
Wehmas, Leah C. [1 ]
Wood, Charles E. [1 ]
Gagne, Remi [2 ]
Williams, Andrew [2 ]
Yauk, Carole [2 ]
Gosink, Mark M. [3 ]
Dalmas, Deidre [4 ]
Hao, Ruixin [5 ]
O'Lone, Raegan [6 ]
Hester, Susan [1 ]
机构
[1] US EPA, Natl Hlth & Environm Effects Res Lab, MD B105-03,109 TW Alexander Dr, Res Triangle Pk, NC 27709 USA
[2] Hlth Canada, Environm Hlth Sci & Res Bur, Ottawa, ON K1A 0K9, Canada
[3] Pfizer Drug Safety R&D, Groton, CT 06340 USA
[4] GlaxoSmithKline, King Of Prussia, PA 19406 USA
[5] DuPont Co Inc, Newark, DE 19714 USA
[6] ILSI Hlth & Environm Sci Inst, Washington, DC 20005 USA
关键词
RNA quality; FFPE; archival resources; RNA integrity number; RNA-sequencing; DIFFERENTIAL EXPRESSION ANALYSIS; GENE-EXPRESSION; DOSE-RESPONSE; KEY EVENTS; FORMALDEHYDE FIXATION; CANCER; MODE; OPTIMIZATION; PROFILES; REMOVAL;
D O I
10.1093/toxsci/kfx278
中图分类号
R99 [毒物学(毒理学)];
学科分类号
100405 ;
摘要
Archival formalin-fixed paraffin-embedded (FFPE) tissue samples offer a vast but largely untapped resource for genomic research. The primary technical issues limiting use of FFPE samples are RNA yield and quality. In this study, we evaluated methods to demodify RNA highly fragmented and crosslinked by formalin fixation. Primary endpoints were RNA recovery, RNA-sequencing quality metrics, and transcriptional responses to a reference chemical (phenobarbital, PB). Frozen mouse liver samples from control and PB groups (n = 6/group) were divided and preserved for 3 months as follows: frozen (FR); 70% ethanol (OH); 10% buffered formalin for 18 h followed by ethanol (18F); or 10% buffered formalin (3F). Samples from OH, 18F, and 3F groups were processed to FFPE blocks and sectioned for RNA isolation. Additional sections from 3F received the following demodification protocols to mitigate RNA damage: short heated incubation with Tris-Acetate-EDTA buffer; overnight heated incubation with an organocatalyst using 2 different isolation kits; or overnight heated incubation without organocatalyst. Ribo-depleted, stranded, total RNA libraries were built and sequenced using the Illumina HiSeq 2500 platform. Overnight incubation (+/- organocatalyst) increased RNA yield > 3-fold and RNA integrity numbers and fragment analysis values by> 1.5-and > 3.0-fold, respectively, versus 3F. Postsequencing metrics also showed reduced bias in gene coverage and deletion rates for overnight incubation groups. All demodification groups had increased overlap for differentially expressed genes (77%-84%) and enriched pathways (91%-97%) with FR, with the highest overlap in the organocatalyst groups. These results demonstrate simple changes in RNA isolation methods that can enhance genomic analyses of FFPE samples.
引用
收藏
页码:535 / 547
页数:13
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