Prep your station and set yourself up for success
Working with RNA can be tricky because of its unstable nature and, to further complicate things, the ubiquitous presence of ribonucleases in cells, tissues, and the environment, can rapidly degrade RNA. To avoid degradation, keep these tips in mind as you get started on your RNA extraction process:
- Clean your bench and pipettors thoroughly with 70% ethanol and 3% hydrogen peroxide, or use our RNase Erase decontamination solution.
- Wear gloves to protect your samples from RNases on your skin
- Use RNase-free reagents, tubes, and tips
- Keep your samples cold throughout your protocol unless it specifically says to perform a step at room temperature or to apply heat
- Work swiftly—prep your station, solutions, and equipment before you startÂ
RNase Erase® decontamination solution, 500 mL
Protect your RNA by completely removing RNase contamination from bench tops, glass and plasticware.
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Learn the Basic Steps of RNA Extraction
There are several different methods of RNA extraction, but they all involve the same basic steps. Depending on the method, the order of the steps (particularly steps 4-6 in Table 1), will change.
Table 1 Basic Steps of RNA Extraction
| Step |
Action |
Description |
| 1 |
Harvest the cells or tissue |
Collecting the source of RNA.
- For bacterial cells, this involves centrifuging the cells and discarding the broth media.
- For a monolayer of mammalian cells, this could simply involve aspirating the media and washing the cells with PBS.
- For tissues, you will need to dissect the target tissue.
|
| 2 |
Lyse the cells |
You can effectively lyse your cells with lysis buffers containing chaotropic agents (e.g., guanidinium isothiocyanate) or through mechanical disruption, such as lysing matrices (or a combination).
The approach you select will heavily depend on your sample type.
Bacterial cells can easily be lysed with buffers, whereas tough tissues will require more aggressive measures.
|
| 3 |
Inactivate RNases |
This is critical for protecting your RNA and can be achieved using chaotropic agents, such as phenol and chloroform.
|
| 4 |
Capture the RNA |
The RNA can be localized to a specific liquid phase during liquid-liquid extraction (e.g., phenol chloroform extraction) or captured through binding to a solid surface, such as silica.
If using a liquid-liquid extraction method, the RNA needs to be precipitated after extraction so that it can be collected using centrifugation. 100% alcohol (e.g., isopropanol or ethanol) is the most commonly used reagent for precipitating nucleic acids.
|
| 5 |
Remove DNA, proteins, and other cellular components |
You can degrade DNA with RNase-free DNase and degrade proteins with proteinase K.
Different protocols introduce these reagents at different times.
Alternatively, you can repeat organic extraction using phenol and chloroform or dissolve the sample in buffers containing guanidinium salts, to remove proteins.
|
| 6 |
Resuspend or elute RNA |
Generally, isolated RNA gets resuspended or eluted in DEPC-treated water or a buffer compatible with downstream applications.
|
| 7 |
Quantitate the RNA and assess the quality |
Evaluate your RNA yield, the concentration of your solution, and the quality and purity of your RNA. This is most often done using UV spectroscopy.
|
| 8 |
Store the purified RNA |
To maintain RNA integrity and prevent degradation, you should keep isolated RNA at -80°C for long-term storage.
|
Lysing Matrices
Get reproducible homogenization with MP Bio’s bead beating tubes and ready-to-use lysing matrices for any sample type.
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Know Your Options—Methods of RNA Extraction
There are several methods of RNA extraction, listed in Table 2, with the most commonly used non-kit-based method being the guanidium-acid-phenol extraction—commonly referred to as TRIzol and TRIreagent (however there are several excellent reagents and commercial kits on the market for the guanidium-acid-phenol extraction method).
Table 2 Common Methods of RNA Extraction
| Methods of RNA Extraction |
Description |
| Guanidium-acid-phenol extraction |
A liquid-liquid extraction method using centrifugation.
RNA remains in an upper aqueous phase and proteins and DNA are separated into a lower phenol phase.
RNA gets precipitated out using alcohol.
|
| Silica technology, glass fiber filters |
Solid-phase extraction often used in commercial kits in the form of column-spin filters.
RNA binds silica (dependent on chaotropic salts), which gets washed and then eluted.
|
| Cesium chloride/cesium triflouroacetate density gradient centrifugation |
A liquid-liquid extraction method using ultracentrifugation to create a CsCl gradient.
RNA gets pelleted, washed, resuspended, and then precipitated with alcohol.
|
| Magnetic bead technology |
Superparamagnetic 20-30 nm particles that can vary in surface material, such as silica, to trap RNA.
An external magnetic field is used to trap the particles through wash and elution steps.
|
| Lithium chloride and urea isolation |
Tissues get homogenised in urea-lithium to precipitate RNA.
Then a phenol-chloroform solution is used to separate proteins from RNA.
Then ethanol is used to precipitate RNA
|
| Lithium chloride (LiCl) precipitation |
LiCl is an alternative to using alcohol for precipitation—and can be advantageous for RNA extraction as it preferentially precipitates RNA compared with DNA.
|
| Oligo(dt)-cellulose column |
A useful column chromatographic method for isolating mRNA or synthetic RNAs with a poly(A) tail by trapping RNA on oligo-dT-cellulose resin through complementary base pairing.
|
RNA-PLUSâ„¢ (phenol solution), 100 mL
For single step RNA isolation with efficiency removal of DNA and proteins. RNAs obtained with RNA-PLUSâ„¢ are not degraded and are free of proteins and DNA.
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Choosing the right RNA isolation method
Choosing the right method early will save you time and sample, but with the large variety of methods and kits available for RNA extraction, the right method may be difficult to identify.
Answering the following questions will help you select the best method of RNA extraction:
- What is your sample type and how difficult is it to lyse?
- What type of RNA do you need to isolate (e.g., miRNAs, tRNAs, total RNA, etc.)?
- How much RNA does your downstream application require?
- How many samples are you processing—should you consider high-throughput methods? Â
- Will certain resuspension solutions interfere with your downstream application?
- Do you need to isolate other molecules from your sample (e.g., proteins or DNA)?
You can obtain high-quality, ready-to-use RNA from virtually any sample with MP Bio’s kits (Table 3), and some of the kits are available for high-throughput needs and have protocols that can be adapted so you can isolate proteins and RNA from a single sample.
Table 3: MP Bio RNA Isolation Kits
| Kit |
Sample type |
Description |
Reference |
| FastRNA Pro Soil-Direct |
Soil/Environmental |
Isolate total RNA from organic matter in soil or from soil supernatants.
The kit removes humic substances and other inhibitors, and efficiently inactivates cellular RNases during homogenization to prevent RNA degradation.
|
Read |
| FastRNA Pro Soil-Indirect |
Soil/Environmental Supernatants |
Read |
| FastRNA ProBlue |
Gram +/- Bacteria |
Intact total RNA is released in the RNAProâ„¢ solution where it is immediately stabilized. The RNAProâ„¢ solution inactivates cellular RNases during cell lysis to prevent RNA degradation. RNA is extracted with chloroform and precipitated with ethanol. DEPC-treated water is provided for re-suspension of total RNA.
|
Read |
| FastRNA ProRed |
Yeast, Fungi |
Read |
| FastRNA Pro Green |
Plants, Animals tissue, Cultured Cells |
Read |
| FastRNAâ„¢ SPIN Kit for Microbes |
Tough-to-lyse Bacterial Cell Cultures |
Isolate total RNA in approximately 15 minutes.
|
Read |
| FastRNAâ„¢ SPIN Kit for Yeast |
Tough-to-lyse Yeast Strains, Fungi and Algae |
Read |
| RapidPure RNA Plant Kit |
Plant Cells, Plant Tissues and Filamentous Fungi |
Isolate total RNA via spin filter columns. Unlike the FastRNA systems, this kit does not use Lysing Matrices to lyse the cells. Use the FastRNA Pro Green kit as an alternative.
|
 |
| RapidPure RNA Tissue Kit |
Human and Animal Tissues |
Isolate and purify high quality total RNA from small amounts of various human and animal tissues. Simultaneously isolation of total RNA and proteins.
Unlike the FastRNA systems, this kit does not use Lysing Matrices to lyse the cells. Use the FastRNA Pro Green kit as an alternative.
|
 |
| MPure Viral RNA Extraction Kit |
Human Biological Specimens |
Isolate viral RNA using a magnetic bead solution.
|
 |
| MPure Total RNA Extraction Kit |
Whole Blood, Blood Cells, Animal Tissue, Plant Tissue, Yeast or Cultured Cells |
Isolate total RNA using a magnetic bead solution.
|
Read |
Isolating RNA using the guanidium-acid-phenol extraction method
This is a common liquid-liquid extraction method, which may take longer than silica-based columns, but often has a higher recovery of RNA. It works by relying on phase separation by centrifugation of an aqueous sample mixed with a solution of phenol and chloroform. After centrifugation, an upper aqueous layer and a lower phenol layer are clearly formed, with the upper layer containing your target RNA.
Guanidium thiocyanate is a chaotropic agent that is a component of trizol and is important in denaturing proteins that may bind to nucleic acids or degrade RNA.
The pH is incredibly important. Low pH, around 4, ensures that only RNA preferentially remains in the aqueous phase while DNA and protein remain in the organic phenol layer. This differs from DNA extraction, which uses a guanidinium thiocyanate-phenol solution with pH to 6 or 7, causing DNA and RNA to partition into the aqueous phase.
Isopropyl alcohol can be added to the aqueous phase (after transferred to a fresh tube) to precipitate RNA. The alcohol disrupts the hydration shells neutralizing the negative phosphate backbone of RNA. Instead of water molecules, positively charged metal salt ions neutralize the negatively charged RNA. The neutral RNA begins to aggregate in the aqueous solution, which gets pelleted using centrifugation. Washing steps with 70% ethanol remove salts and DEPC (Diethylpyrocarbonate)-treated water is used to redissolve the RNA pellet.
Why DEPC water? DEPC nonspecifically inhibits RNase by reacting with amine, hydroxy, and thiol groups within enzymes.
RNAPro Solution, 2 x 27.5 mL
Efficiently isolate total RNA from any type of plant and animal tissue or cultured cells, microbes, or soil and environmental samples. Recent publication
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General Method of RNA Extraction from Bacterial Cells
- Pellet bacterial cells that were growing overnight by centrifuging for 2 minutes at 12,000xgÂ
- Decant luria broth supernatant
- Resuspend the pellet in RNA-PLUSâ„¢ (comparable to TRIzol) and lyse cells by pipetting several times. Make sure you get the entire pellet—sometimes residual pellet can linger at the bottom of your tube, which will reduce your yield.Â
- Centrifuge for 10 minutes at 4°C at 12,000xg
- Transfer the supernatant to a fresh tube (Do not invert the tube, it might leak)
- Add chloroform, shake vigorously (or vortex), and incubate for 3 minutes at room temperature
- Centrifuge for 15 minutes at 12,000xg. Now you should see an upper, colorless aqueous phase (this contains your RNA) and a lower reddish phenol phase (this contains contaminating proteins).
- Transfer the upper aqueous phase to a clean RNase-free tube, careful not to transfer any phenol phase
- Add 100% isopropyl alcohol and incubate for 10 minutes at room temperature to precipitate the RNA
- Centrifuge at 12,000g for 10 minutes at 4°CÂ
- Discard the supernatantÂ
- Wash the pellet with 70%-80% ethanol (invert the tube a few times)
- Centrifuge at 4°C for 5 minutes at 7500xg
- Discard the ethanolÂ
- Air dry the pellet for roughly 10 minutes at room temperature
- Resuspend the pellet in DEPC-treated water (or your choice of buffer)
Quantitate your RNA and assess the quality
Before using your RNA, you need to know how much you have and that it’s worth using. The most common method for quantitating RNA is UV spectroscopy.
Quantity: A260 of 1.0 is roughly 40 µg/mL single-stranded RNA (assuming the pH is ~7.5)
Quality: A260/A280 of 1.8-2.1 indicates highly purified RNA
Keep in mind that this method will not differentiate between RNA and DNA, so you should consider treating your samples with RNase-free DNase
Store your purified RNA
You’ve successfully isolated RNA! Now you just need to store it to keep it safe and ready to use for your next experiment.
We recommend storing RNA at –80°C in single-use aliquots to avoid using damaged RNA from freeze-thaw cycles and to help prevent RNase contamination.
