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Quantitating RNA
RNA quantitation is an important
and necessary step prior to most RNA analysis methods. Here we
discuss three common methods used to quantitate RNA and tips
for optimizing each of these methods.
UV Spectroscopy
The traditional method for assessing RNA
concentration and purity is UV spectroscopy. The absorbance of
a diluted RNA sample is measured at 260 and 280 nm. The nucleic
acid concentration is calculated using the Beer-Lambert law, which
predicts a linear change in absorbance with concentration (Figure
1).
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| Figure 1. Beer-Lambert
Law for Calculating UV Absorbance by Nucleic Acid. |
| BLANK/DILUENT |
A260/A280 RATIO |
| DEPC-treated water (pH 5-6) |
1.60 |
| Nuclease-free water (pH 6-7) |
1.85 |
| TE (pH 8.0) |
2.14 |
|
| Figure 2. Effects
of pH on A260/A280 Ratio. |
Using this equation, an A260 reading
of 1.0 is equivalent to ~40 µg/ml single-stranded RNA.The
A260/A280 ratio is used to assess RNA purity.
An A260/A280 ratio of 1.82.1 is indicative
of highly purified RNA.
UV spectroscopy is the most widely
used method to quantitate RNA. It is simple to perform, and UV spectrophotometers
are available in most laboratories. The method does have several
drawbacks, but they can be minimized by following these tips:
Tips for Optimizing Performance
- Because this method does not discriminate
between RNA and DNA, it is advisable to first treat RNA samples
with RNase-free DNase to remove contaminating DNA.
- Other contaminants such as residual proteins
and phenol can interfere with absorbance readings, so care must
be taken during RNA purification to remove them.
- Sample readings are made in quartz cuvettes.
Dirty cuvettes and dust particles cause light scatter at 320 nm
which can impact absorbance at 260 nm. Since neither proteins nor
nucleic acids absorb at 320 nm, perform a background correction
by making readings from a blank (diluent only) at 320 nm, as well
as 260 nm and 280 nm.
- The A260/A280 ratio is
dependent on both pH and ionic strength. As pH increases, the A280 decreases
while the A260 is unaffected. This results in an increasing
A260/A280 ratio (Wilfinger, et. al 1997).
Because water often has an acidic pH, it can lower the A260/A280 ratio.
We recommend using a buffered solution with a slightly alkaline
pH, such as TE (pH 8.0), as a diluent (and as a blank) to assure
accurate and reproducible readings. An example of the variation
in A260/A280 ratio at different pH values
is shown in Figure 2.
- Make sure your RNA dilution is within the linear
range of your spectrophotometer. Usually absorbance values should
fall between 0.1 and 1.0. Solutions that are outside this range
cannot be measured accurately. Generally the greatest error occurs
at lower concentrations.
Because an A260 of 0.1
corresponds to ~4 µg/ml RNA, it is often impractical to use
UV spectroscopy to quantitate RNA isolated from small samples that
will have lower concentrations once diluted. Fortunately, there are
alternative methods for accurately quantitating small amounts of
RNA two are described below.
Fluorescent Dyes
Certain fluorescent dyes, such as RiboGreen® (Molecular
Probes), exhibit a large fluorescence enhancement when bound to
nucleic acids. As little as 1 ng/ml of RNA can be detected and
quantitated using RiboGreen with a standard fluorometer, fluorescence
microplate reader, or filter fluorometer.
To accurately quantitate RNA, unknowns
are plotted against a standard curve produced with a sample of known
concentration, usually based on its absorbance at 260 nm. The linear
range of quantitation with RiboGreen can extend three orders of magnitude
(1 ng/ml to 1 µg/ml) when two different dye concentrations are
used. Furthermore RiboGreen® assays are relatively insensitive
to non-nucleic acid contaminants commonly found in nucleic acid preparations,
so that linearity is maintained.
Tips for Optimizing Performance
- Because RiboGreen does not discriminate between
RNA and DNA, it is advisable to treat RNA samples with RNase-free
DNase to remove contaminating DNA.
- The RiboGreen reagent can adsorb to the sides
of tubes. This can be minimized by preparing solutions in non-stick,
nuclease-free polypropylene plasticware.
- Protect the RiboGreen reagent from photodegradation
by wrapping the container with foil and use the reagent within
several hours of preparation.
- Avoid repeated freeze-thaw cycles of
RNA standards. This can cause strand-scission of the RNA, resulting
in decreased dye binding. In addition, nucleic acids can adsorb
to tubes with repeated freeze-thaw cycles. This phenomenon becomes
more pronounced at lower concentrations.
Agilent 2100 Bioanalyzer
The Agilent 2100 bioanalyzer uses a combination
of microfluidics, capillary electrophoresis, and fluorescent dye
that binds to nucleic acid to evaluate both RNA concentration and
integrity. An RNA reference standard (the RNA 6000 Ladder Cat#
7152; Ambion) and a microfluidics chip (The RNA Lab Chip; Agilent
Technologies) are also required. The RNA 6000 Ladder is composed
of six RNAs ranging in size from 0.26 kb. The ladder and
samples are loaded in designated wells on the RNA Lab Chip. Size
and mass information is provided by the fluorescence of RNA molecules
as they move through the channels of the chip. The instrument software
automatically compares the peak areas from unknown RNA samples
to the combined area of the six RNA 6000 Ladder RNA peaks to determine
the concentration of the unknown samples. The RNA 6000 Nano System
has a broad dynamic range and can quantitate between 25500
ng/ml of RNA with a covariance of ~10%.
Perhaps the most powerful feature
of the Agilent 2100 bioanalyzer is its ability to provide information
about RNA integrity. As each RNA sample is analyzed, the software
generates both a gel-like image and an electropherogram (Figure 3).
When analyzing total RNA, the areas under the 18S and 28S ribosomal
RNA peaks are used to calculate the ratio of these two major ribosomal
RNA species and these data are displayed along with quantitation
data on individual electropherograms (Figure 3a). Significant changes
in the ratios of the 18S and 28S ribosomal RNA peaks are indicative
of degraded RNA.
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| Figure 3. Agilent
2100 Bioanalyzer Electropherograms of RNA Samples. A. Electropherogram
of a Total RNA Sample. Total
RNA (100 ng) was analyzed on an Agilent 2100 bioanalyzer.
The resulting electropherogram shows the characteristic signature
of a high quality total RNA sample. B. Electropherogram
of Amplified aRNA Sample. Total
RNA 2 µg corresponding to 60 ng mRNA) was amplified
using the MessageAmp aRNA Kit (Ambion Cat# 1750) resulting
in (90 µg aRNA, a 1500 fold amplification. The aRNA
(900 ng) was analyzed on an Agilent 2100 bioanalyzer. The
resulting electropherogram shows the classic output of a
high quality aRNA sample. |
In addition to its usefulness for
analysis of total RNA, the bioanalyzer is also a superior tool for
analyzing mRNA and amplified aRNA (antisense RNA) integrity. Intact
mRNA and aRNA profiles consist of a broad distribution of signal,
with the bulk of the RNA usually falling between 1 and 2 kb, though
this will vary from tissue to tissue (Figure 3b). A significant shift
of the profile towards lower molecular weights is indicative of poor
RNA integrity.
Tips for Optimizing Performance
- The area of the peaks derived from the RNA
6000 Ladder is used as a mass standard for unknowns, so accurate
quantitation of your unknowns is dependent on careful handling
of this standard. We recommend that the RNA 6000 Ladder be thoroughly
mixed and carefully pipetted to reduce error. For best performance,
the standard should be aliquoted into non-stick, nuclease-free
tubes to avoid multiple freeze-thaw cycles of a single stock tube.
- Quantitation is affected by ionic strength
of the sample, which can quench fluorescence in RNA samples. Therefore,
when possible, RNA should be suspended in nuclease-free water to
minimize differences between the RNA 6000 Ladder and the sample
to be measured. If this is not possible, be aware that the unknown
concentration may be underestimated.
- Generally, we find that some 23S and 28S rRNAs
do not migrate according to their molecular weights. For example,
mammalian 28S rRNA, 4.8 kb in length, consistently migrates just
ahead of the 4 kb peak in the RNA 6000 Ladder. This is likely due
to
the highly structured nature of 23S and 28S rRNAs.
- Although this assay has a broad linear range
(~25 ng500 ng) overloading the chip with RNA can affect performance
of the RNA Lab Chip. For consistent results, we recommend loading
50 ng250 ng of RNA.
- The fluorescent dye is light sensitive, so
store dye concentrate and working solutions away from light; e.g.
wrap tubes in foil.
- Follow the manufacturer's recommendations for
maintenance of the electrodes and the priming station. Poor Lab
Chip Loading (priming) and formation of salt bridges between electrodes
are common causes of poor assay performance.
References
1. Wilfinger WW, Mackey K, and Chomczynski
P (1997) Effect of pH and ionic strength on the spectrophotometric
assessment of nucleic acid purity. Biotechniques 22:474481.
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Ordering Information
For prices and availability, please contact our Customer Service Department.
| Cat# |
Product Name |
Size |
| AM2222 |
DNase I (RNase-free) (2 U/µl) |
2000 U |
| AM7152 |
RNA 6000 Ladder |
3 x 20 µl |
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