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在RNA提取中替代β-巯基乙醇。

Replacing β-mercaptoethanol in RNA extractions.

作者信息

Mommaerts Kathleen, Sanchez Ignacio, Betsou Fay, Mathieson William

机构信息

Integrated Biobank of Luxembourg, L-1210 Luxembourg, Luxembourg.

Integrated Biobank of Luxembourg, L-1210 Luxembourg, Luxembourg.

出版信息

Anal Biochem. 2015 Jun 15;479:51-3. doi: 10.1016/j.ab.2015.03.027. Epub 2015 Apr 2.

Abstract

RNA extractions are potentially compromised in terms of both yield and quality by ribonucleases (RNases). The pungent and toxic reducing agent β-mercaptoethanol (β-ME), therefore, is commonly added to the biospecimen's lysis buffer to aid in RNase deactivation. Using different tissue types (liver tissue, kidney tissue, and cell pellets), extraction kits (RNeasy Mini Kit, Illustra RNA Spin Mini Kit, and PureLink Mini Kit), RNA quality assays (RNA integrity numbers [RINs] and quantitative real-time polymerase chain reaction [qRT-PCR]), yield assessments, and in vitro functional RNase assays (RNaseAlert Kit), we demonstrate that β-ME should be replaced by the less toxic dithiothreitol (DTT) alternative.

摘要

核糖核酸酶(RNases)可能会在产量和质量方面对RNA提取造成潜在影响。因此,通常会在生物样本的裂解缓冲液中添加刺鼻且有毒的还原剂β-巯基乙醇(β-ME),以帮助使RNase失活。我们使用不同的组织类型(肝脏组织、肾脏组织和细胞沉淀)、提取试剂盒(RNeasy Mini试剂盒、Illustra RNA Spin Mini试剂盒和PureLink Mini试剂盒)、RNA质量检测方法(RNA完整性数值[RINs]和定量实时聚合酶链反应[qRT-PCR])、产量评估以及体外功能性RNase检测方法(RNaseAlert试剂盒),证明β-ME应由毒性较小的二硫苏糖醇(DTT)替代。

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