Nonradioactive Detection of Small RNAs Using Digoxigenin-Labeled Probes

Tomassi, Ariel Hernán; Gagliardi, Delfina; Cambiagno, Damián Alejandro; Manavella, Pablo Andrés

info:eu-repo/semantics/publishedVersion

Fecha

2017

Registro en:

Tomassi, Ariel Hernán; Gagliardi, Delfina; Cambiagno, Damián Alejandro; Manavella, Pablo Andrés; Nonradioactive Detection of Small RNAs Using Digoxigenin-Labeled Probes; Humana Press; 1640; 2017; 199-210

978-1-4939-7164-0

http://hdl.handle.net/11336/108116

CONICET Digital

CONICET

https://repositorioslatinoamericanos.uchile.cl/handle/2250/4324056

Autor

Tomassi, Ariel Hernán

Gagliardi, Delfina

Cambiagno, Damián Alejandro

Manavella, Pablo Andrés

Institución

Consejo Nacional de Investigaciones Científicas y Tecnológicas (Argentina)

Resumen

Small RNAs have been traditionally detected and quantified using small RNA blots, a modified Northern blot technique. The small RNAs are size-fractionated from the rest of the cellular RNA molecules by polyacrylamide gel electrophoresis and transferred by blotting onto a positively charged membrane. A radiolabeled probe was then traditionally used to detect a specific small RNA in the cellular pool. Small RNA blotting is a relatively simple, inexpensive approach to visualize small RNAs without artifacts. However, the radioactive labeling of the probe is sometimes an impediment, especially due to the requirement of specialized facilities. Here we describe a sensitive and simple method to detect and quantify small RNAs using digoxigenin-based nonradioactive RNA blots.

Materias

Polyacrylamide electrophoresis

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