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首页> 外文期刊>Journal of Applied Phycology >A method for extracting a high-quality RNA from Symbiodinium sp
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A method for extracting a high-quality RNA from Symbiodinium sp

机译:一种从Symbiodinium sp中提取高质量RNA的方法

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摘要

Good quality RNA is essential for a range of analyses including microarray and gene expression studies. A number of methods for RNA extraction from symbiotic dinoflagellates were assessed for their ability to recover a high-quality RNA applicable for evaluation of gene expression profiles. The recovery and quality of the obtained RNA were evaluated with respect to UV light absorbance profiles and automated microcapillary electrophoretic RNA separation. A modified RNA extraction procedure that combines two existing commercial kits, Trizol and Qiagen RNeasy kits, was efficiently employed for the recovery of a high-quality RNA under specific homogenization conditions. Cell homogenization using glass beads at the speed of 4,500 rpm for up to 6 min resulted in a good RNA recovery and preserved RNA integrity. A high-quality RNA obtained following the described procedure was successfully applied in reverse transcriptase-polymerase chain reaction (PCR) and in quantitative PCR studies. Gene expression profiles were changed with RNA extraction procedure, with the highest transcript numbers at precise conditions of cell homogenization. RNA samples with RNA integrity number values from 6 and above were recommended for downstream applications. This sequence of RNA isolation and RNA evaluation represents a methodological improvement required for functional genomic studies in dinoflagellates.
机译:高质量的RNA对于包括微阵列和基因表达研究在内的各种分析至关重要。评估了从共生鞭毛藻中提取RNA的多种方法,它们具有回收可用于评估基因表达谱的高质量RNA的能力。关于紫外线吸收曲线和自动微毛细管电泳RNA分离,评估了获得的RNA的回收率和质量。结合了两个现有的商用试剂盒Trizol和Qiagen RNeasy试剂盒的改良RNA提取程序可有效地用于在特定的均质化条件下回收高质量的RNA。使用玻璃珠以4,500 rpm的速度进行细胞均质化长达6分钟,可实现良好的RNA回收并保留RNA完整性。按照上述步骤获得的高质量RNA已成功应用于逆转录聚合酶链反应(PCR)和定量PCR研究中。基因表达谱用RNA提取程序改变,在精确的细胞均质条件下具有最高的转录数。建议将RNA完整性编号值大于等于6的RNA样品用于下游应用。 RNA分离和RNA评估的这一序列代表了鞭毛藻功能基因组研究所需的方法学改进。

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