RNA Isolation Protocol
互联网
1004
RNA Isolation Protocol
(Revised 5-15-2003)
Stabilize RNA
Start with 15 ml E. coli Culture containing 7.undefined 109 cells (OD600 = 0.2 Dilute cells or scale up)
-
Pipet 30 ml of RNAProtect Bacteria Reagent (Qiagen) into a 50ml polypropylene conical tube.
-
Pipet 15 ml culture into the tube. Mix immediately by vortexing for 5second. Incubate for 5min at room temperature.
-
Centrifuge for 10min at 5800g( 4500rpm for H-6000A rotor in SORVALL RC-3B centrifuge)
-
Decant the supernatant, and leave tubes inverted on a paper towel for 10s.
-
Freeze the pellet with EtOH/Dye Ice mix.
-
The pellet can be stored at -20°C up to 2 weeks, or -70°C for up to 4 weeks.
Isolation RNA
-
Dilute 2ul of Proteinase K into 300ul of Tissue and Cell Lysis solution for each sample.
-
Resuspend cell pellet by the Lysis solution and mix thoroughly. Transfer mix to 1.5ml tube.
-
Incubate at 65°C for 45min, and vortex every 15min.
-
Place the sample on ice for 5min.
-
Add 150ul of MPC protein Precipitation Reagent to 300ul of lysed sample and vortex mix for 10sec.
-
Spin for 10min 4°C at max speed in a microcentrifuge. Transfer the supernant to a clean tube.
-
Add 50ul of MPC protein Precipitation Reagent and repeat above step.
-
Add 500ul isopropanol to the recovered supernatant, invert the tube 30-40 times.
-
Pellet the RNA by centrifugation at 4°C for 10min in a microcentrifuge.
-
Carefully pour off the isopropanol without dislodging the RNA pellet. Remove all of the residual isopropanol with a pipet. Air dry 10-15min.
Removal of contaminating DNA
-
Dilute 10ul of RNAse-Free DNAse I up to 200ul with 1x DNAse Buffer for each sample.
-
Completely resuspend the nucleic acid pellet in 200ul of DNAse I solution.
-
Incubation at 37deg;C for 45min
-
Add 200ul of 2x T and C lysis solution, vortex mix for 5 seconds
-
Add 200ul of MPC reagent vortex mix 10seconds, place on ice 5min.
-
Pellet the debris by centrifugation for 10min at 4°C, >10,000g in a microcentrifuge.
-
Add 50ul of MPC reagent and repeat 5 and 6 (but this time spin 20min).
-
Add 600ul isopropanol to the recovered supernatant, invert the tube 30-40 times.
-
Pellet the RNA by centrifugation at 4°C for 10min in a microcentrifuge.
-
Carefully pour off the isopropanol without dislodging the RNA pellet.
-
Rinse with 75% EtOH (DEPC H2 O), being careful to not dislodge the pellet. Centrifuge 5min at 4°C
-
Remove all of the residual EtOH with a pipet. Air dry 10-15min.
-
Resuspend the nucleic acid in 52ul RNAse-free water.
Storage, Quantitation and Determination of Quality of RNA
-
Electrophoresis on 1% Agarose gel with 1ul sample.
-
Dilute 1ul sample to 100ul with TE(10mM Tris.HCl pH 8, 1mM EDTA), and measure A260 and A280 with a spectrophotometer.. Alternatively 1ul sample can be used to measure A260 and A280 on a Nanodrop ND-1000 Spectrophotometer without dilution.
-
Concentration of RNA sample = 40 x A260 x 100 (Dilution factor) (ug/ml)
-
A260/A280 Ratio = A260/A280, ranging from 1.7 to 2.1
-
Add 100ul EtOH (2 volume) and 5ul 3M NaOAC (1/10 volume), store at -20°C
Regents
-
RNAProtect Bacteria Reagent Qiagen
-
MasterPure RNA Isolation Kit Epicentre
Note: This protocol was adapted from the original Qiagen and Epicentre protocols
