Preparation of RNA Gel Blots
-
Last Update: 2021-03-04
-
Source: Internet
-
Author: User
Search more information of high quality chemicals, good prices and reliable suppliers, visit
www.echemi.com
RNA gel blots (often referred to as Northern gel blots) are frequently used in the analysis of gene expression, for example when investigating specificity of gene expression, quantification of transcription, and analysis of RNA processing. Electrophoresis of RNA through agarose gels for blotting requires complete denaturation of the RNA. A number of denaturants have been used, including glyoxal and dimethyl sulfoxide (
1
), methylmercuric hydroxide (
2
), and formaldehyde (
3
). The following protocol described by Fourney et al. (
4
), uses formaldehyde as the denaturant but at a lower concentration than previously suggested. This allows direct visualization of the RNA without the need for staining and washing of the gel. The buffer system used is
MOPS
, which unlike Tris-HCl is suitable for use with formaldehyde
see
Note 1 ). The RNA is then transferred to a nylon membrane by capillary blotting for subsequent hybridization. Mol-wt standards can be used to estimate transcript size if required.
This article is an English version of an article which is originally in the Chinese language on echemi.com and is provided for information purposes only.
This website makes no representation or warranty of any kind, either expressed or implied, as to the accuracy, completeness ownership or reliability of
the article or any translations thereof. If you have any concerns or complaints relating to the article, please send an email, providing a detailed
description of the concern or complaint, to
service@echemi.com. A staff member will contact you within 5 working days. Once verified, infringing content
will be removed immediately.
