gDNA RNA Clean Up Protocol
Wesley Elias Bhering Barrios, Débora Gonçalves Gouveia
Abstract
Protocol used to eliminate DNA fragments and gDNA from purified RNA and to remove impurities from the sample.
Before start
*** Use only sterile RNAse-Free tubes - AM12425 - or sterile Axygen RNAse Free microtubes.
*** All calculations should be performed before the beginning of the procedure, since reagents and samples have high added value.
Steps
Procedure
Starting with the 27 uL left over from each sample, add another 62 uL of RNAse-Free H2O at room temperature to all samples;
Prepare DNAse Mix I and add 11 uL of the Mix per sample;
10 uL of 10X DNAse I Buffer * No. of samples;
1 uL of DNAse I * No. of samples;
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11 uL * No. of samples * 1.06
*** Final reaction volume = 100 uL, adjust the final volume if less than 100 uL.
Incubate the samples in the thermomixer at 37º C, without shaking, for 20 minutes;
Add 1 uL of RNAse Free 0.5M EDTA pH 8.0 to each sample;
Incubate at 75°C for 10 minutes;
Prepare the RNA Precipitation Mix:
150 uL Water treated with 0.1% DEPC * No. of samples
100 uL 4M Ammonium Acetate * No. of samples
350 uL Ethanol 200 proof Molecular Biology Grade (99.45%) * No. of samples
____
600 uL of Mix * No. of samples * 1.06
Add 600 uL of the RNA Precipitation Mix to each sample and INVERT 20X using a microtube rack;
Incubate at -80°C for 30 minutes or overnight at -20°C;
Centrifuge at 4°C for 20 minutes at 13,000 RPM;
Discard the supernatant with the aid of pipette tips;
Add 300 uL of 75% Molecular Biology Grade Ethanol prepared with 0.1% DEPC-treated Milli-Q Water (only add to wash the pellet, and vortex for less than 1 second);
Centrifuge at 4°C for 5 minutes at 13,000 RPM;
Discard the supernatant with the aid of pipette tips;
Add 300 uL of 75% Ethanol for Molecular Biology prepared with 0.1% DEPC-treated Milli-Q Water (only add to wash the pellet, and vortex for less than 1 second);
Centrifuge at 4°C for 7 minutes at 13,000 RPM;
Discard the supernatant with the aid of pipette tips;
Leave the tubes open in a 1.5 mL microtube rack in the fume hood for 5 minutes;
Resuspend the pellet in 20 uL of 0.1% DEPC-treated Milli-Q Water at 60 °C from tube to tube, homogenizing moderately for 30 seconds per sample (use P20 in 15 uL volume);
Run 1.5% agarose gel in 1X TAE buffer + 5% bleach (80 V - 80 min);
***The electrophoresis vat should be thoroughly cleaned with RNAse Zap + Distilled Water and fresh running buffer should be added, the gel polymerization tray should be thoroughly cleaned and the gel should be made with fresh buffer to avoid RNA degradation.
If the RNA is intact (identify 18S and 28S rRNA bands at 2Kb and 4.8Kb), determine the concentration and quality parameters (A260/A230 and A260/A280) of the sample in the spectrophotometer/nanodrop;
If RNA is used in more sensitive applications, quantify in Qubit;
Store the samples in the ultra-freezer (-80 ºC) for up to 6 months.
