Odogwu Nkechi Martina, Jang Jin Sung, Albertson Sabrina, Hagen Clinton, Rasmussen Boyd, Saji Oommen, Nelson Timothy J
Program for Hypoplastic Left Heart Syndrome, Mayo Clinic Rochester, Rochester, Minnesota, United States of America.
Genome Analysis Core, Medical Genome Facility, Center for Individualized Medicine, Mayo Clinic Rochester, Rochester, Minnesota, United States of America.
PLoS One. 2024 Dec 26;19(12):e0315098. doi: 10.1371/journal.pone.0315098. eCollection 2024.
Archived FFPE cardiac tissue specimens are valuable for molecular studies aimed at identifying biomarkers linked to mortality in cardiovascular disease. Establishing a reliable and reproducible RNA extraction method is critical for generating high-quality transcriptome sequences for molecular assays. Here, the efficiency of four RNA extraction methods: Qiagen AllPrep DNA/RNA method (Method QP); Qiagen AllPrep DNA/RNA method with protocol modification on the ethanol wash step after deparaffinization (Method QE); CELLDATA RNA extraction (Method BP) and CELLDATA RNA extraction with protocol modifications on the lysis step (Method BL) was compared on 23 matching FFPE cardiac tissue specimens (n = 92).In comparing RNA quality metrics across FFPE RNA extract, nucleic acids extracted deploying Method QE and QP produced the highest RNA yield. However, Method QE outperformed Method QP as more extract from Method QE had DV 200 values above 30%. Both method BL and BP produced similar range of RNA purity and yield but more extract from Method BL had DV 200 values above 30% compared to Method BP. When accessing distribution value, Method BL outperformed Methods BP, QE, and QP as more extracts from Method BL had DV 200 values above 30% compared to other methods (PDV200<0.001; Kruskal-Wallis). Method QE outperformed other methods in terms of RNA yield. RNA extracts from Method QE, characterized by high RNA yield, achieved sequencing results comparable to those from Method BL, characterized by high DV200 values. Our findings reveal that optimizing protocols can yield higher-quality RNA, facilitating the exploration of more disease conditions with high-resolution transcriptome profiling.
存档的福尔马林固定石蜡包埋(FFPE)心脏组织标本对于旨在识别与心血管疾病死亡率相关生物标志物的分子研究具有重要价值。建立一种可靠且可重复的RNA提取方法对于生成用于分子检测的高质量转录组序列至关重要。在此,我们在23对匹配的FFPE心脏组织标本(n = 92)上比较了四种RNA提取方法的效率:Qiagen AllPrep DNA/RNA方法(方法QP);在脱石蜡后的乙醇洗涤步骤进行方案修改的Qiagen AllPrep DNA/RNA方法(方法QE);CELLDATA RNA提取方法(方法BP)以及在裂解步骤进行方案修改的CELLDATA RNA提取方法(方法BL)。在比较FFPE RNA提取物的RNA质量指标时,采用方法QE和QP提取的核酸产生的RNA产量最高。然而,方法QE优于方法QP,因为方法QE提取的更多样本的DV 200值高于30%。方法BL和BP产生的RNA纯度和产量范围相似,但与方法BP相比,方法BL提取的更多样本的DV 200值高于30%。在评估分布值时,方法BL优于方法BP、QE和QP,因为与其他方法相比,方法BL提取的更多样本的DV 200值高于30%(PDV200<0.001;Kruskal-Wallis检验)。方法QE在RNA产量方面优于其他方法。以高RNA产量为特征的方法QE提取的RNA,其测序结果与以高DV200值为特征的方法BL相当。我们的研究结果表明,优化方案可以产生更高质量的RNA,有助于通过高分辨率转录组分析探索更多疾病情况。
