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Excess primer degradation by Exo?I improves the preparation of 3′ cDNA ligation-based sequencing libraries

机译:EXO的过量引物降解ααβ-I改善了3'CDNA连接的测序文库的制备

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摘要

RNA sequencing library construction using single-stranded ligation of a DNA adapter to 3′ ends of cDNAs often produces primer–adapter byproducts, which compete with cDNA–adapter ligation products during library amplification and, therefore, reduces the number of informative sequencing reads. We find that Escherichia coli Exo I?digestion efficiently and selectively removes surplus reverse transcription primer and thereby reduces the primer–adapter product contamination in 3′ cDNA ligation-based sequencing libraries, including small RNA libraries, which are typically similar in size to the primer–adapter products. We further demonstrate that Exo I treatment does not lead to trimming of the cDNA 3′ end when duplexed with the RNA template. Exo I digestion is easy to perform and implement in other protocols and could facilitate a more widespread use of 3′ cDNA ligation for sequencing-based applications.
机译:使用DNA适配器的单链连接至CDNA的3'末端的RNA测序文库施工通常产生引物 - 适配器副产物,其在图书馆放大期间与cDNA-Adapter连接产品进行竞争,因此减少了信息读数的次数。 我们发现大肠杆菌exo I?有效地消化并选择性地去除剩余逆转录引物,从而减少3'CDNA结扎的测序文库中的引物衔接剂产品污染,包括小RNA文库,其通常与引物的尺寸相似 - 产品。 我们进一步证明EXO I治疗不会导致与RNA模板双工时CDNA 3'结束。 EXO I消化易于在其他方案中进行和实现,并且可以促进更广泛使用3'CDNA连接以进行排序的应用。

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