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灌注和解剖小鼠腮腺以及从鼠类和人类腮腺组织中分离高质量RNA的分步方案。

Step-by-step protocol to perfuse and dissect the mouse parotid gland and isolation of high-quality RNA from murine and human parotid tissue.

作者信息

Watermann Christoph, Valerius Klaus Peter, Wagner Steffen, Wittekindt Claus, Klussmann Jens Peter, Baumgart-Vogt Eveline, Karnati Srikanth

机构信息

Institute for Anatomy and Cell Biology, Medical Cell Biology, Justus-Liebig-University, Giessen, Germany.

Department of Otorhinolaryngology, Head and Neck Surgery, Justus-Liebig-University, Giessen, Germany.

出版信息

Biotechniques. 2016 Apr 1;60(4):200-3. doi: 10.2144/000114404. eCollection 2016 Apr.

Abstract

Macroscopic identification and surgical removal of the mouse parotid gland is demanding because of its anatomic location and size. Moreover, the mouse parotid gland contains high concentrations of RNases, making it difficult to isolate high-quality RNA. So far, appropriate methods for optimal perfusion-fixation and dissection of mouse parotid glands, as well as the isolation of high quality RNA from this tissue, are not available. Here we present a simple, optimized, step-by-step surgical method to perfuse and isolate murine parotid glands. We also compared two common RNA extraction methods (RNeasy Mini Kit versus TRIzol) for their yields of high-quality, intact RNA from human and murine parotid gland tissues that were either snap-frozen or immersed in RNAlater stabilization solution. Mouse parotid tissue that was perfused and immersed in RNAlater and human samples immersed in RNAlater exhibited the best RNA quality, independent of the isolation method.

摘要

由于小鼠腮腺的解剖位置和大小,对其进行宏观识别和手术切除颇具难度。此外,小鼠腮腺中含有高浓度的核糖核酸酶,这使得分离高质量的RNA变得困难。到目前为止,尚无适用于小鼠腮腺最佳灌注固定和解剖以及从该组织中分离高质量RNA的方法。在此,我们介绍一种简单、优化的分步手术方法,用于灌注和分离小鼠腮腺。我们还比较了两种常见的RNA提取方法(RNeasy Mini试剂盒与TRIzol),以评估它们从速冻或浸入RNAlater稳定溶液的人和小鼠腮腺组织中提取高质量完整RNA的产量。灌注后浸入RNAlater的小鼠腮腺组织以及浸入RNAlater的人类样本,无论采用何种分离方法,均表现出最佳的RNA质量。

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