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3 ' READS plus , a sensitive and accurate method for 3 ' end sequencing of polyadenylated RNA

机译:3'READS plus,一种灵敏而准确的多腺苷酸化RNA 3'末端测序方法

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摘要

Sequencing of the 3' end of poly(A)(+) RNA identifies cleavage and polyadenylation sites (pAs) and measures transcript expression. We previously developed a method, 3' region extraction and deep sequencing (3'READS), to address mispriming issues that often plague 3' end sequencing. Here we report a new version, named 3'READS+, which has vastly improved accuracy and sensitivity. Using a special locked nucleic acid oligo to capture poly(A)(+) RNA and to remove the bulk of the poly(A) tail, 3'READS+ generates RNA fragments with an optimal number of terminal A's that balance data quality and detection of genuine pAs. With improved RNA ligation steps for efficiency, the method shows much higher sensitivity (over two orders of magnitude) compared to the previous version. Using 3'READS+, we have uncovered a sizable fraction of previously overlooked pAs located next to or within a stretch of adenylate residues in human genes and more accurately assessed the frequency of alternative cleavage and polyadenylation (APA) in HeLa cells (similar to 50%). 3'READS+ will be a useful tool to accurately study APA and to analyze gene expression by 3' end counting, especially when the amount of input total RNA is limited.
机译:聚(A)(+)RNA的3'端测序确定了切割和聚腺苷酸化位点(pAs),并测量了转录表达。我们以前开发了一种方法,即3'区域提取和深度测序(3'READS),以解决经常困扰3'末端测序的引物错误问题。在这里,我们报告了一个名为3'READS +的新版本,该版本大大提高了准确性和灵敏度。 3'READS +使用特殊的锁定核酸寡核苷酸捕获poly(A)(+)RNA并去除大部分poly(A)尾巴,从而生成具有最佳末端A数量的RNA片段,从而平衡数据质量和检测真正的pA。通过改进的RNA连接步骤以提高效率,与以前的版本相比,该方法显示出更高的灵敏度(超过两个数量级)。使用3'READS +,我们发现了人类基因中腺苷酸残基旁边或其中一段片段中先前被忽略的pA的相当大一部分,并更准确地评估了HeLa细胞中交替切割和聚腺苷酸化(APA)的频率(大约50% )。 3'READS +将成为准确研究APA并通过3'末端计数来分析基因表达的有用工具,尤其是在输入总RNA数量有限的情况下。

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