RNA extraction using trizol method

RNA Extraction Process Explained

Importance of RNA Extraction

• The video discusses the significance of RNA extraction in various applications, such as detecting viral RNA using quantitative PCR and analyzing gene expression.

• High-quality RNA is crucial for successful outcomes in techniques like RNA sequencing and quantitative PCR, making the extraction process vital.

TriZol Extraction Method

• The most common method for RNA extraction is the TriZol extraction method, which utilizes a monophasic solution of phenol and guanidine isothiocyanate.

• Cells or tissues are collected in an endof tube; cells can be broken open by pipetting, while tissues require homogenization for effective extraction.

Homogenization and Phase Separation

• After homogenizing tissue samples with a pestle, chloroform is added to create a liquid-liquid interface that separates components during centrifugation.

• Following centrifugation, the aqueous phase contains RNA while the organic phase holds proteins and lipids.

Precipitation and Washing of RNA

• Isopropanol is added to precipitate the RNA from the aqueous solution; this step allows visualization of a pellet if present.

• The pellet can be washed with ethanol before being dissolved in DEPC-treated water to ensure integrity and prevent RNase contamination.

Quality Assessment of Extracted RNA

• Agarose gel electrophoresis checks RNA quality by visualizing 28S, 18S, and 5S rRNA bands; intact RNA indicates successful extraction.

• Quantification methods include using a bioanalyzer or Nanodrop; A260/A280 ratios help assess purity. An RIN value above 9 is preferred for sequencing purposes.