Quantitative analysis of noncoding RNA from paired fresh and formalin-fixed paraffin-embedded brain tissues

被引:0
作者
Yehui Lv
Shiying Li
Zhihong Li
Ruiyang Tao
Yu Shao
Yijiu Chen
机构
[1] Sichuan University,West China School of Basic Medical Sciences & Forensic Medicine
[2] Academy of Forensic Science,Shanghai Key Laboratory of Forensic Medicine
[3] Shanghai University of Medicine & Health Science,School of basic medical sciences
来源
International Journal of Legal Medicine | 2020年 / 134卷
关键词
Forensic science; Forensic pathology; Formalin-fixed paraffin-embedded (FFPE); RNA; Noncoding RNA (ncRNA); Real-time quantitative polymerase chain reaction (RT-qPCR);
D O I
暂无
中图分类号
学科分类号
摘要
Formalin-fixed paraffin-embedded (FFPE) tissues are commonly used both clinically and in forensic pathology. Recently, noncoding RNA (ncRNA) has attracted interest among molecular medical researchers. However, it remains unclear whether newly identified ncRNAs, such as long noncoding RNA (lncRNA) and circular RNA (circRNA), remain stable for downstream molecular analysis in FFPE tissues. Here, we assessed the feasibility of using autoptic FFPE brain tissues from eight individuals to perform quantitative molecular analyses. Selected RNA targets (9 mRNAs and 15 ncRNAs) with different amplicon lengths were studied by RT-qPCR in paired fresh and FFPE specimens. For RNA quality assessment, RNA purity and yield were comparable between the two sample cohorts; however, the RNA integrity number decreased significantly during FFPE sampling. Amplification efficiency also displayed certain variability related with amplicon length and RNA species. We found molecular evidence that short amplicons of mRNA, lncRNA, and circRNA were amplified more efficiently than long amplicons. With the assistance of RefFinder, 5S, SNORD48, miR-103a, and miR-125b were selected as reference genes given their high stability. After normalization, we found that short amplicon markers (e.g., ACTB mRNA and MALAT1 lncRNA) exhibited high consistency of quantification in paired fresh/FFPE samples. In particular, circRNAs (XPO1, HIPK3, and TMEM56) presented relatively consistent and stable expression profiles in FFPE tissues compared with their corresponding linear transcripts. Additionally, we evaluated the influence of prolonged storage time on the amplification of gene transcripts and found that short amplicons still work effectively in archived FFPE biospecimens. In conclusion, our findings demonstrate the possibility of performing accurate quantitative analysis of ncRNAs using short amplicons and standardized RT-qPCR assays in autopsy-derived FFPE samples.
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页码:873 / 884
页数:11
相关论文
共 445 条
[1]  
Higuchi R(1993)Kinetic PCR analysis: real-time monitoring of DNA amplification reactions Biotechnology (N Y) 11 1026-1030
[2]  
Fockler C(2005)Real-time PCR for mRNA quantitation Biotechniques 39 75-85
[3]  
Dollinger G(2014)Insights into RNA structure and function from genome-wide studies Nat Rev Genet 15 469-479
[4]  
Watson R(2016)From the RNA world to the clinic Science 352 1417-1420
[5]  
Wong ML(2016)Non-coding RNAs: classification, biology and functioning Adv Exp Med Biol 937 3-17
[6]  
Medrano JF(2013)Long non-coding RNAs: a new frontier in the study of human diseases Cancer Lett 339 159-166
[7]  
Mortimer SA(2013)Circular RNAs are a large class of animal RNAs with regulatory potency Nature 495 333-338
[8]  
Kidwell MA(2015)Forensic application of microRNA-706 as a biomarker for drowning pattern identification Forensic Sci Int 255 96-101
[9]  
Doudna JA(2017)Estimation of the human postmortem interval using an established rat mathematical model and multi-RNA markers Forensic Sci Med Pathol 13 20-27
[10]  
Sullenger BA(2017)Cell death-associated ribosomal RNA cleavage in postmortem tissues and its forensic applications Mol Cell 40 410-417
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