TBS-380
Mini-Fluorometer Method for
RNA Quantitation Using
RiboGreen®
1. INTRODUCTION
The Turner
BioSystems TBS-380 Mini-Fluorometer in combination with Molecular Probes'
RiboGreen® RNA quantitation reagent provides a method for
ultrasensitive quantitation of RNA in solution. Detecting and quantitating
small amounts of RNA is extremely important for a wide variety of molecular
biology procedures. These include measuring yields of in vitro transcribed RNA, measuring RNA concentrations before performing Northern
blot analysis, S1 nuclease assays, RNase protection assays, cDNA library
preparation, and reverse transcription PCR and differential display PCR.
The conventional
technique for measuring nucleic acid concentration is the determination
of absorbance at 260 nm (A260). The major disadvantages of
the A260 method are the relative large contribution of proteins and free
nucleotides to the signal, the inability to distinguish between DNA and
RNA, the interference caused by contaminants commonly found in nucleic
acid preparations, and the relative insensitivity of the assay (an A260 of 0.1 corresponds to a 4 µg/mL
RNA solution). The use of fluorescent nucleic acid stains alleviates many
of these problems.
The RiboGreen® RNA quantitation assay used in conjunction with the TBS-380 Mini-Fluorometer
can detect as little as 1 ng/mL RNA (Figure 1), exceeds the sensitivity
of ethidium bromide-based fluorometric assays1 by 200-fold and A260 measurements by 1000-fold. The linear quantitation range extends over
two and half orders of magnitude in RNA concentration, using two dye concentrations.
Using one concentration of RiboGreen® reagent and the recommended
assay protocol, researchers can quantitate 25 ng/mL to 500 ng/mL RNA.
By diluting the RiboGreen® reagent 10-fold further, 1 ng/mL
to 50 ng/mL RNA can be quantitated. Linearity is maintained in the presence
of several compounds commonly found to contaminate nucleic acid preparations.
Although the RiboGreen® reagent also binds to DNA, pretreatment
of mixed samples with DNase can be used to generate an RNA-selective assay.
2. MATERIALS
REQUIRED
·
TBS-380 Mini-Fluorometer (P/N 3800-003).
· 10x10 mm square methacrylate cuvettes (P/N 7000-959).
· Minicell Adaptor Kit (P/N 3800-928).
· RiboGreen® RNA Quantitation Kit, supplied by Molecular
Probes, Inc., Eugene, OR (catalog number R-11490). The kit contains 1
mL of RiboGreen® RNA quantitation reagent stock solution
in DMSO, 25 mL of 20X TE assay buffer (200 mM Tris-HCl, 20 mM EDTA, pH
7.5 in DEPC (diethylpyrocarbonate-treated water) and 1 mL (supplied as
5 x 200 µL)
of 100 µg/mL
16S and 23S ribosomal RNA standard (from E. coli), in TE buffer.
The kit contents are sufficient for 200 high-range (20 ng/mL to 1 µg/mL)
RNA assays using 2.0 mL samples in 10x10 mm cuvettes. RiboGreen® RNA Quantitation Reagent (1 mL in DMSO) is also available from Molecular
Probes as a separate item (catalog number R-11491). Handling, storage
and the use of the reagents should be performed in accordance with the
product information sheet supplied by Molecular Probes, Inc.
· Nuclease-free water (see Section 3.2, below).
3. EXPERIMENTAL
PROTOCOL
3.1 Overview
Two different dye concentrations are required to achieve the full linear
dynamic range of the RiboGreen® RNA quantitation assay.
Different working solutions of RiboGreen® reagent are prepared
for the high-range assay (25 ng/mL to 500 ng/mL RNA) and the low-range assay (1 ng/mL to 50 ng/mL RNA), as described below in Section 3.3.
3.2 Assay
Buffer Preparation
TE assay buffer (10 mM Tris-HCl, 1 mM EDTA, pH 7.5) is used for diluting
the RiboGreen® reagent and the RNA samples. It is imperative
that the TE buffer is free of contaminating nucleases and nucleic acids.
Clean disposable gloves should be worn during handling and preparation
of all materials and solutions. All solutions should be prepared in sterile
disposable plasticware or nuclease-free glassware, using nuclease-free
pipettes. The 20X TE buffer that is included in the RiboGreen® RNA Quantitation Kit is nuclease-free and nucleic acid-free. This buffer
is also available from Molecular Probes, Inc. as a separate item (catalog
number T-11493). Prepare the 1X TE working solution by diluting the concentrated
buffer 20-fold with nuclease-free water. Nuclease-free water should be
prepared by treating distilled, deionized water with 0.1% diethylpyrocarbonate
(DEPC), incubating for several hours at 37°C
and autoclaving for at least 15 minutes at 15 PSI inch to sterilize and
eliminate DEPC. Caution: DEPC is a suspected carcinogen and should
be handled with care. Compounds containing amines, such as Tris, will
react rapidly with DEPC and should be added to DEPC treated water only
after DEPC is removed by heating. Removal of DEPC by heating is also important
to prevent carboxyethylation of the RNA sample.2
3.3 Reagent
Preparation
On the day of the experiment, prepare a 2X working solution of the RiboGreen® reagent by diluting an aliquot of the concentrated DMSO stock solution
into 1X TE. If performing the high-range assay, dilute 200-fold.
For example, to prepare enough working solution to assay 20 samples in
2 mL volumes, add 100 µL
RiboGreen® RNA quantitation reagent to 19.9 mL 1X TE. If
performing the low-range assay, dilute 2000-fold. For example,
to prepare enough working solution to assay 20 samples in 2 mL volumes,
add 10 µL
RiboGreen® RNA quantitation reagent to 20.0 mL 1X TE. Prepare
these solutions in sterile, disposable, polypropylene plasticware rather
than glassware, as the reagent may adsorb to glass surfaces. Protect the
working solutions from light by covering them with foil or placing them
in the dark, as the RiboGreen® reagent is susceptible to
photodegradation.
For best results, these solutions should be used within a few hours
of their preparation.
3.4 RNA
Standard Curves
3.4.1 Prepare a 2 µg/mL
solution of RNA in 1X TE using nuclease-free plasticware. Determine the
RNA concentration on the basis of absorbance at 260 nm (A260)
in a cuvette with a 1 cm pathlength; an A260 of 0.05 corresponds to 2 µg/mL
RNA. The 16S and 23S ribosomal RNA standard, provided at 100 µg/mL
in the RiboGreen® RNA Quantitation Kit, can simply be diluted
50-fold in 1XTE to make the 2 µg/mL
working solution. For example, 40 µL
of the RNA standard mixed with 1.96 mL of TE will be sufficient for the
standard curve described below. It is sometimes preferable to prepare
the standard curve with purified RNA similar to the type being assayed.
In general, equivalent amounts of single-stranded RNA from different sources
produce approximately equal fluorescence intensity readings. The assay
remains linear in the presence of several compounds that commonly contaminate
nucleic acid preparations, including nucleotides, salts, urea, ethanol,
chloroform, detergents, proteins and agarose. However the fluorescence
intensity may be affected (see Molecular Probes product information sheet
MP11490 for details) and therefore the RNA solution used to prepare the
standard curve should be treated the same way as the experimental samples
and should contain similar levels of such compounds.
3.4.2 For the high-range standard curve, make a series of RNA standard
solution at 2X final concentration by diluting the 2 µg/mL
RNA solution into disposable cuvettes or nuclease-free plastic test tubes
for transfer to Minicell cuvettes (see table 1).
2X
RNA solution concentration (ng/mL ) |
Volume
of the 2X RNA solution (mL) |
Volume
of the 2X high-range working
solution (mL) |
Final
RNA Concentration in RiboGreen® Assay (ng/mL)
|
1000 |
1 |
1 |
500 |
200 |
1 |
1 |
100 |
100 |
1 |
1 |
50 |
50 |
1 |
1 |
25 |
0 |
1 |
1 |
blank |
Table
1. High-range RNA standard curve for 10x10 mm
cuvette.
For the low-range standard curve, make a series of RNA standard solution at 2X final concentration
by diluting the 2 µg/mL RNA solution into disposable cuvettes or
nuclease-free plastic test tubes for transfer to Minicell cuvettes (see
table 2).
2X
RNA solution concentration (ng/mL ) |
Volume
of the 2X RNA solution (mL) |
Volume
of the 2X low-range working
solution (mL) |
Final
RNA Concentration in RiboGreen® Assay (ng/mL)
|
100 |
1 |
1 |
50 |
50 |
1 |
1 |
25 |
20 |
1 |
1 |
10 |
10 |
1 |
1 |
5 |
2 |
1 |
1 |
1 |
0 |
1 |
1 |
blank |
Table
2. Low-range RNA standard curve for 10x10 mm cuvette.
3.4.3 Mix equal volume of the 2X working solution of RiboGreen® reagent (prepared in Section 3.3) with each 2X RNA standard solution.
The high-range working solution (200-fold dilution of stock) should
only be used for performing the high-range assay and the low-range working solution (2000-fold dilution of stock) should only be used for
performing the low-range assay. Mix well and incubate for 2 to
5 minutes at room temperature, protected from light. Be sure to add enough
volume into the cuvettes. The minimum volume is 2 mL for 10x10 mm cuvette
and 50 µL
for Minicell cuvette.
3.4.4 Select the BLUE channel of the TBS-380 Mini-Fluorometer.
Calibrate the fluorometer using the sample containing the highest concentration
of RNA [Note: For optimal detection sensitivity, separate calibrations
should be carried out for the high range and low range assays]. Measure
the fluorescence of the remaining samples. The TBS-380 Mini-Fluorometer
will give a direct concentration read out, and data may be used to generate
a standard curve of reading versus RNA concentration.
Figure 1. High-range (A) and low-range (B) ribosomal RNA
standard assays performed using RiboGreen® RNA Quantitation
Reagent and the TBS-380 Mini-Fluorometer. Separate instrument calibrations
were carried out for the two assay ranges.
3.5 Sample
Analysis
3.5.1 Dilute each unknown RNA samples in 1X TE to a desired volume
(1.0 mL for 10x10 mm cuvette or 25-100 µL
for Minicell). It may be useful to prepare several dilutions of each experimental
sample. Large dilutions of the experimental sample may serve to diminish
the interfering effect of certain contaminants. However, extremely small
sample volumes should be avoided because they are difficult to pipet accurately.
In addition, the level of assay contaminants should be kept as uniform
as possible throughout an experiment, to minimize sample-to-sample signal
variation. For example, if a series of RNA samples contain widely differing
salt concentrations, they cannot be compared to a single standard curve.
To avoid this problem, simply adjust the concentration of contaminants
to be the same in all samples, if possible. See Section 3.6 for information
on eliminating DNA from the sample.
3.5.2 Add equal volume of the 2X working solution of the RiboGreen® reagent (prepared in Section 3.3) to each sample. Incubate for 2 to 5
minutes at room temperature, protected from light.
3.5.3 Measure the fluorescence of each sample using the same instrument
calibration conditions as used to generate the standard curve (see 3.4.4).
3.6 Eliminating
DNA from Samples
RiboGreen® reagent also binds to DNA. Fluorescence in samples
that is due to RiboGreen® reagent binding to DNA can be
eliminated by pre-treating the sample with RNase-free DNase, ensuring
that the entire sample fluorescence is due to dye bound to RNA.
3.6.1 Prepare 10X DNase digestion buffer: nuclease-free 200 mM Tris-HCl, pH
7.5, containing 100 mM MgCl2 and 20 mM CaCl2.
3.6.2 Add 0.11 sample volume of 10X DNase digestion buffer to each DNA-containing
sample (for example, to a 9 mL sample, add 1 mL 10X buffer).
3.6.3 Add about 5 units of RNase-free DNase I per mg of DNA thought to be in
the sample.
3.6.4 Incubate the sample at 37°C
for 90 minutes.
3.6.5 Dilute the sample at least 10-fold into TE to diminish effects of the
digestion buffer salts on the RiboGreen® assay procedure.
3.6.6 Perform the RiboGreen® assay as described above.
4. REFERENCES
1. Anal Biochem
17, 100 (1966)
2. Sambrook, J., Fritsch, E.F. and Maniatis, T., Molecular Cloning:
A Laboratory Manual, Second Edition, Cold Spring Harbor Laboratory
Press (1989).
5. PATENT
& TRADEMARK INFORMATION
RiboGreen
is a registered trademark of Molecular Probes, Inc. RiboGreen® RNA Quantitation Reagent is covered by current or pending U.S. and foreign
patents.
6. ABOUT MOLECULAR PROBES, INC.
Orders for
Molecular Probes' products may be placed by:
Phone: (541) 465-8338 or
Toll-Free: (800) 438-2209 (U.S. & Canada)
Fax: (541) 344-6504 or
E-mail: order@probes.com
Mailing Address:
Molecular Probes, Inc.
PO Box 22010
Eugene, OR 97402-0414
U.S.A.
Information
on the scientific and technical back-ground of Molecular Probes' products
is available from the Technical Assistance Department by:
Phone: (541)
465-8353
Fax: (541) 465-4593
Web: www.probes.com
E-Mail: tech@probes.com
7. ABOUT TURNER BIOSYSTEMS, INC.
Orders for
Turner BioSystems' products may be placed by:
Phone: (408)
636-2400
Toll Free: (888) 636-2401 or
Fax: (408) 737-7919
Contact us
via our contact
form
Internet: www.turnerbiosystems.com
Mailing Address:
Turner BioSystems, Inc.
645 N. Mary Avenue
Sunnyvale, CA 94085
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