Total RNA Isolation and cDNA synthesis from Bixa orellana bark

P. Santosh, S. B. Arakera
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Abstract

Annatto is one of the important natural food colourant widely used in dairy industry. Quality RNA in large quantity is often required in the analysis of gene expression. RNA extraction from samples collected from woody plants is generally complex, and becomes the main limitation to study gene expression, particularly in crops like Bixa orellana . Standard RNA extraction protocols are time consuming, laborious and cannot be adapted for high throughput functional analysis. Therefore a simple and effective protocol for extraction of high quality total RNA from bark tissue of woody stem was achieved using the RNeasy plant mini kit (Qiagen, USA). The extracted RNA was successfully converted into double-stranded cDNA using the SMATer cDNA synthesis kit (Clontech, USA) which is based on the S witching M echanism A t 5’ End of R NA T ranscript (SMART) technology. The integrity of the total RNA used for synthesizing double stranded cDNA was assessed agarose gel electrophoresis and by PCR. As expected, the PCR product contained the full coding sequence plus 69 and 196 bp of 5’ and 3’ UTRs respectively. The double-stranded cDNA was used successfully for creating a SSH cDNA library. The cDNA could also be useful for a number of other applications like cDNA library construction, EST analysis, RACE and Next Generation Sequencing (NGS).
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苦参树皮总RNA的分离及cDNA的合成
红木是一种重要的天然食用色素,广泛应用于乳制品行业。在基因表达分析中,往往需要大量高质量的RNA。从木本植物采集的样本中提取RNA通常是复杂的,并且成为研究基因表达的主要限制,特别是在Bixa orellana等作物中。标准RNA提取方案耗时,费力,不能适应高通量功能分析。因此,使用RNeasy植物迷你试剂盒(Qiagen, USA)实现了从木本茎的树皮组织中提取高质量总RNA的简单有效的方案。利用SMATer cDNA合成试剂盒(Clontech, USA)成功地将提取的RNA转化为双链cDNA,该试剂盒基于RNA t转录物的5 '端S开关M机制(SMART)技术。通过琼脂糖凝胶电泳和PCR检测合成双链cDNA总RNA的完整性。与预期的一样,PCR产物包含完整的编码序列,分别加上69 bp和196 bp的5 '和3 ' utr。利用该双链cDNA成功构建了SSH cDNA文库。该cDNA还可用于cDNA文库构建、EST分析、RACE和下一代测序(NGS)等其他应用。
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