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Picofluor Handheld Fluorometer Method for
DNA Quantitation Using PicoGreen®
1. INTRODUCTION
PicoGreen dsDNA Quantitation Reagent is an ultra-sensitive fluorescent nucleic
acid stain for quantitating double-stranded DNA (dsDNA) in molecular biological
procedures such as cDNA synthesis for library production and DNA fragment
purification for subcloning, as well as applications, such as quantitating
DNA amplification products1,2 and primer extension assays.3,4
The most commonly used technique for measuring nucleic acid concentration
is the determination of absorbance at 260 nm (A260) The major
disadvantages of the absorbance method are the large relative contribution
of nucleotides, single-stranded nucleic acids and proteins to the signal,
the interference caused by contaminants commonly found in nucleic acid preparations,
the inability to distinguish between DNA and RNA, and the relative insensitivity
of the assay (an A260 of 0.1 corresponds to a 5 µg/mL dsDNA
solution). Hoechst (bis-benzimide) dyes are sensitive fluorescent nucleic
acid stains that circumvent many of these problems. The Hoechst 33258 Dye
- based assay is somewhat selective for dsDNA, does not show significant
fluorescence enhancement in the presence of proteins and allows the detection
and quantitation of DNA concentrations as low as 5.0 ng/mL DNA.5
The Picofluor™ Handheld Fluorometer used in conjunction with
Molecular Probes' PicoGreen dsDNA Quantitation Reagent enables researchers
to quantitate as little as 1 ng/mL of dsDNA. This sensitivity exceeds that
achieved with the Hoechst 33258 Dye. The standard PicoGreen assay protocol
is also simpler than the Hoechst 33258 method, because a single concentration
of the PicoGreen Reagent allows detection over the full dynamic range of
the assay. In order to obtain the full dynamic range with Hoechst-based
assays, two different dye concentrations are recommended. In contrast, the
linear detection range of the PicoGreen assay in the Picofluor Fluorometer
extends four orders of magnitude in DNA concentration - from 1 ng/mL to
1000 ng/mL with a single dye concentration (see Figures 1 and 2). This linearity
is maintained in the presence of several compounds commonly found to contaminate
nucleic acid preparations, including salts, urea, ethanol, chloroform, detergents,
proteins and agarose. The assay protocol has been developed to minimize
the fluorescence contribution of RNA and single-stranded DNA (ssDNA). Using
the PicoGreen dsDNA Quantitation Reagent and the Picofluor Fluorometer,
researchers can quantitate dsDNA in the presence of equimolar concentrations
of ssDNA and RNA with minimal effect on the quantitation results.
Figure 1 . DNA Standard calibration
plot.
2. MATERIALS REQUIRED
- Picofluor™ Fluorometer with
blue optical configuration (P/N 8000-003 or 8000-004)
- 10 X 10 mm methacrylate fluorescence
cuvettes (P/N 7000-959)
- PicoGreen dsDNA Quantitation Reagent,
supplied by Molecular Probes, Inc., Eugene, Oregon, catalog number P-7581.
A single 1-mL unit of the reagent concentrate is sufficient for 200
assays using an assay volume of 2 mL and the protocol described in section
3. Handling, storage and use of the reagent should be performed in accordance
with the product information sheet supplied by Molecular Probes, Inc.
3. EXPERIMENT PROTOCOL
3.1 Reagent Preparation
The PicoGreen dsDNA Quantitation Reagent is supplied as a 1-mL concentrated
dye solution in anhydrous dimethylsulfoxide (DMSO). On the day of the
experiment, prepare an aqueous working solution of the PicoGreen Reagent
by making a 1:200 dilution of the concentrated DMSO solution in 10 mM
Tris-HCl, 1 mM EDTA, pH 7.5 (TE). To prepare enough working solution to
assay 20 samples, add 100 µL PicoGreen dsDNA Quantitation Reagent
to 20.0 mL TE. Preparing this solution in a plastic container is recommended,
as the reagent may adsorb to glass surfaces. Protect the working solution
from light by covering it with foil or placing it in the dark, as the
PicoGreen Reagent is susceptible to photodegradation. For best results,
this solution should be used within a few hours of its preparation.
3.2 DNA Standard Curve
3.2.1 Prepare a 2 µg/mL stock solution of dsDNA in TE. Determine
the DNA concentration on the basis of absorbance at 260 nm (A260) in a
cuvette with a 1-cm pathlength; an A260 of 0.04 corresponds
to 2 µg/mL dsDNA solution. Calf thymus DNA is commonly used for
a standard curve, although any purified dsDNA preparation may be used.
It is preferable to prepare the standard curve with DNA similar to the
type being assayed; long or short linear DNA fragments for quantitating
similar-sized restriction fragments; plasmid for quantitating plasmid
DNA. However, most linear dsDNA molecules have been found to yield approximately
equivalent signals, regardless of fragment length. The PicoGreen assay
remains linear in the presence of several compounds that commonly contaminate
nucleic acid preparations, although the signal intensity may be affected.
Thus, to serve as an effective control, the dsDNA 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. To generate
a single-replicate, five-point standard curve from 1 ng/mL to 1000 ng/mL,
proceed to step 3.2.2.
Note: Only one standard is necessary
for proper calibration. Additional concentrations are optional and may
be useful for checking the linearity of the assay.
3.2.2 For the DNA standard curve, dilute the 2 µg/mL DNA
stock solution into acrylic cuvettes as shown in Table 1. Then add 1.0
mL of the aqueous working solution of PicoGreen Reagent (prepared in section
3.1) to each cuvette. Mix well and incubate for 2 to 5 minutes at room
temperature, protected from light.
Table 1. Protocol for preparing standard curve.
3.2.3 After incubation, calibrate in the Picofluor Fluorometer.
Press "STD VAL" and enter "999" for the highest standard
(1000 ng/mL). Press the "CAL" button and then "Enter".
Next, insert blank from chart above and press "Enter". After
blank is read insert the most fluorescent sample (1 µg/mL DNA) and
press "Enter".
3.2.4 Measure the fluorescence of
the remaining samples. To equalize any photobleaching effects, insert
samples into the fluorometer for approximately equal time periods. The
readout is the actual concentration of the sample as it relates to the
standard unit of measure (ng/mL).
4. REFERENCES
1. Nucleic Acids Res. 24, 2623 (1996)
2. BioTechniques 21, 372 (1996)
3. BioTechniques 21, 664 (1996)
4. Proc. Natl. Acad. Sci. USA 93, 6091 (1996)
5. Anal. Biochem. 102, 344 (1980)
6. Molecular Cloning: A Laboratory Manual, Second Edition, J. Sambrook,
E.F. Fritsch and T. Maniatis, Cold Spring Harbor Laboratory Press, Cold
Spring Harbor, New York (1989).
5. WARNINGS AND PRECAUTIONS
The PicoGreen dsDNA Quantitation Reagent is the subject of patent applications
filed by Molecular Probes, Inc. and is not available for resale or other
commercial uses without a specific agreement from Molecular Probes, Inc.
PicoGreen is a registered trademark of Molecular Probes, Inc.
6. ABOUT MOLECULAR PROBES, INC.
Orders for Molecular Probes' products may be placed by:
Phone: (541) 465-8338 or
Toll-Free: (800) 438-2209 in the U.S. and Canada
Fax: (541) 344-6504 or
Toll-Free: (800) 438-0228 in the U.S. and Canada
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
background of Molecular Probes' products is available from the Technical
Assistance Dept:
Phone: (541) 465-8353
Fax: (541) 465-4593
E-mail: tech@probes.com
Internet: http://www.probes.com
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