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Achieving high throughput sequencing of a cDNA library utilizing an alternative protocol for the bench top next-generation sequencing system

机译:利用台式下一代测序系统的替代方案实现cDNA文库的高通量测序

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The development of next-generation sequencing (NGS) technologies has provided novel tools for genome analysis and expression profiling. A high throughput cDNA sequencing method using a bench top next-generation sequencing system, GS Junior, is now available. Here, we used an alternative protocol to the standard method for generating the cDNA library. This protocol can decrease the number of processing steps to manipulate RNA when constructing a cDNA library from an RNA sample, and does not require mRNA isolation from total RNA. Thus it can decrease the risk of RNA degradation and the cost for preparing a cDNA library. Also, the efficiency of sequencing data obtained with this approach is comparable to the standard method as verified by sequencing characteristics and expression levels of the reference gene glyceraldehyde-3-phosphate dehydrogenase (GAPDH)
机译:下一代测序(NGS)技术的发展为基因组分析和表达谱分析提供了新颖的工具。现在提供使用台式下一代测序系统GS Junior的高通量cDNA测序方法。在这里,我们使用了标准方法的替代方案来生成cDNA文库。当从RNA样品构建cDNA文库时,此协议可以减少操作RNA的处理步骤,并且不需要从总RNA中分离出mRNA。因此,它可以降低RNA降解的风险和制备cDNA文库的成本。同样,通过这种方法获得的测序数据的效率可与标准方法相媲美,该标准方法已通过参考基因3-磷酸甘油醛脱氢酶(GAPDH)的测序特性和表达水平验证

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