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melRNA-seq for Expression Analysis of SINE RNAs and Other Medium-Length Non-Coding RNAs

机译:Melrna-SEQ用于正弦RNA和其他中长非编码RNA的表达分析

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Small interspersed elements (SINEs) are transcribed by RNA polymerase III (Pol III) to produce RNAs typically 100–500 nucleotides in length. Although their RNA abundance can be evaluated by Northern blotting and primer extension, the nature (sequence, exact length, and genomic origin) of these RNAs cannot be revealed by these methods. Moreover, mRNA sequencing (mRNA-seq) is not able to distinguish bona fide SINE RNAs or SINE sequences present in longer transcripts. To elucidate the abundance, source loci, and sequence nature of SINE RNAs, we established a deep sequencing method, designated as melRNA-seq (medium-length RNA-seq), which can determine whole-length RNA sequences. Total RNA samples were treated with 5′ pyrophosphohydrolase (RppH), which allowed ligation of an RNA adaptor to the 5′ end of intact SINE RNAs. Similarly, another adaptor was ligated to the 3′ end, followed by reverse transcription, PCR amplification, size selection, and single-end deep sequencing. The analysis of two biological replicates of RNAs from mouse spermatogonia showed high reproducibility of SINE expression data both at family and locus levels. This new method can be used for quantification and detailed sequence analysis of medium-length non-coding RNAs, such as rRNA, snRNA, tRNAs, and SINE RNAs. Further, its dynamic range is much wider than Northern blotting and primer extension.
机译:小帧间的元素(凸片)由RNA聚合酶III(POL III)转录,以产生通常100-500个核苷酸的RNA。尽管它们的RNA丰度可以通过Northern印迹和引物延伸来评估这些RNA的性质(序列,精确长度和基因组)不能通过这些方法揭示。此外,mRNA测序(mRNA-SEQ)不能区分真绒正弦RNA或在较长的转录物中存在的正弦序列。为了阐明正弦RNA的丰度,源基因座和序列性质,我们建立了一种深度测序方法,称为MelRNA-SEQ(中长RNA-SEQ),其可以确定全长RNA序列。用5'焦磷酸盐酶(RPPH)处理总RNA样品,其使RNA适配器连接到完整正弦RNA的5'末端。类似地,将另一个适配器连接到3'末端,然后逆转录,PCR扩增,尺寸选择和单端深序。对小鼠精子寄生虫的两种生物学重复的分析表明,家庭和基因座水平都显示出正弦表达数据的高再现性。该新方法可用于中长非编码RNA的量化和详细序列分析,例如RRNA,SNRNA,TRNA和正弦RNA。此外,其动态范围比Northern印迹和底漆延伸得多。

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