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一种无需无核糖核酸酶条件的非放射性原位杂交方法。

A non-radioactive in situ hybridization method that does not require RNAse-free conditions.

作者信息

Tongiorgi E, Righi M, Cattaneo A

机构信息

International School for Advanced Studies (SISSA), Neuroscience Program, Trieste, Italy.

出版信息

J Neurosci Methods. 1998 Dec 1;85(2):129-39. doi: 10.1016/s0165-0270(98)00123-x.

Abstract

This report describes a quick and versatile method to perform non-radioactive in situ hybridization in which none of the hybridization steps are performed under RNAse-free conditions. This study demonstrates that in situ hybridization can be performed without an RNAse-free environment provided that the concentration of RNAse introduced during the experiment does not reach 0.1 microg/ml, a concentration that is unlikely to be achieved through an accidental contamination. Moreover, evidence is provided that the only step sensitive to RNAse degradation is the pretreatment since degradation during the hybridization step can not occur due to a very efficient protective effect exerted by formamide. Finally, our data suggest that endogenous RNAse activity might be readily neutralized through paraformaldehyde fixation. A feature of this method is the strong fixation that ensures a perfect tissue preservation, even at level of the fine structure of the cell processes. The method allows a uniform tissue penetration by sodium periodate and sodium borohydride treatment and can be easily used in combination with diaminobenzidine immunohistochemistry for double labeling experiments.

摘要

本报告描述了一种快速且通用的非放射性原位杂交方法,其中没有一个杂交步骤是在无RNA酶条件下进行的。本研究表明,只要实验过程中引入的RNA酶浓度未达到0.1微克/毫升(通过意外污染不太可能达到该浓度),原位杂交就可以在无RNA酶环境下进行。此外,有证据表明,对RNA酶降解敏感的唯一步骤是预处理,因为由于甲酰胺发挥的非常有效的保护作用,杂交步骤期间不会发生降解。最后,我们的数据表明,通过多聚甲醛固定可能很容易中和内源性RNA酶活性。该方法的一个特点是强力固定,即使在细胞突起的精细结构水平也能确保完美的组织保存。该方法通过高碘酸钠和硼氢化钠处理可实现组织的均匀渗透,并且可以很容易地与二氨基联苯胺免疫组织化学结合用于双重标记实验。

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