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Increasing Sensitivity in
Northern Analysis with RNA Probes
Note: The pointers in this technical bulletin
presuppose the use of standard 50% formamide hybridization solutions.
However, if ULTRAhyb™, Ambion's ultrasensitive hybridization
buffer, is used, the differences in sensitivity between single-stranded
RNA and double-stranded DNA probes are not significant. ULTRAhyb
is now a part of every NorthernMax™ Kit that Ambion sells.
Using RNA probes in Northern analyses results
in significantly greater sensitivity as compared to double-stranded
DNA probes. This fact has been recognized in the literature (1,
2, 3), by other manufacturers of labeling and detection kits, and
by data generated here at Ambion. The 8 to 10-fold increase in
sensitivity provided by switching to an RNA probe will substantially
reduce exposure times and increase the ability to detect rare mRNAs,
often avoiding the need for poly(A) RNA isolation.
Concern About the Use of RNA Probes
Many people are aware of the increased
sensitivity afforded by RNA probes, but have been reluctant to
use them for one or more of the following reasons:
- Fear of degradation of probe molecules
during hybridization
- Reports of high background or heavy
cross-hybridization
- A sense that making transcription templates
or doing in vitro RNA labeling is too difficult and time consuming.
All of these concerns, in fact, are valid when
using standard protocols for Northern analysis and in vitro transcription.
As RNA analysis has become more commonplace, however, better understanding
of the properties of RNA, the availability of ribonuclease-free
enzymes and reagents, and the publication of improved protocols
are beginning to change these common misconceptions.
RNA Probe Synthesis
Making RNA probes is now an easy and straightforward
procedure. Virtually all modern cloning vectors have one or more
bacteriophage promoters (T7, T3, or SP6) outside the multiple cloning
site. To prepare these plasmid templates for in vitro transcription
of the antisense strand (for hybridization to cellular RNA) the
plasmid simply needs to be linearized by restriction enzyme digestion
at or near the 5' end of the insert. If PCR products are to be
labeled, or cDNA/gene inserts are cloned into a vector without
appropriate promoter sites, a simple PCR strategy can be used to
add a phage promoter sequence directly to existing PCR products
or plasmid constructs.
Current in vitro transcription procedures, like that used in Ambion's
MAXIscript™ Kit, are single-tube reactions providing ready-to-use,
high-specific activity probes for Northern analysis in an hour
or less.
Northern Blot Protocols
Improved Northern protocols that take into
account
- The very high thermodynamic stability
of RNA:RNA duplexes
- Hybridization buffers with RNA-appropriate
stabilizing and blocking agents and
- The availability of RNase-free reagents
allow the routine use of RNA probes in
Northerns with no more difficulty or chance of failure than that
associated with DNA probes.
Considerations
When performing Northern analyses using
RNA probes rather than DNA probes, we recommend that several
adjustments be made to obtain the best results. These include:
- The type of membrane used
- RNA-appropriate hybridization buffer
- Elevated hybridization and wash temperatures,
and
- Probe "stripping" techniques.
Ambion offers kits for performing Northern analyses:
NorthernMax™ (Cat #1940)
and NorthernMax-Gly™ (Cat #1946).
Commonly used Northern blotting reagents are also provided as stand-alone
products. Both kits and reagents have been optimized for use with
radiolabeled and nonisotopic RNA probes, and incorporate the following
suggestions.
Preventing Degradation of RNA During Hybridization
Degradation of the probe (and immobilized mRNA)
is prevented by using nuclease-free reagents in the hybridization
buffer. We do not see any apparent degradation of RNA probes, even
at relatively high temperatures, if the hybridization reagents
are certified RNase-free. If nuclease contamination is shown to
be a problem, it is much more likely that nucleases inadvertently
introduced in "home-made" reagents (particularly BSA, a component
of Denhardt's reagent), are responsible. Northern hybridization
buffers, such as Ambion's NorthernMax Pre-hybridization/Hybridization
Buffer and ULTRAhyb, a component of the NorthernMax Complete Northern
Blotting kit, contain only reagents that are certified nuclease-free.
Preventing Cross-Hybridization
Cross-hybridization is significantly reduced
by conducting hybridization at a much higher, and more appropriate,
stringency than previously recommended for RNA probes. The common "rule
of thumb" for RNA probes was to hybridize at 42°C in 50% formamide
and 1 M salt. For the average RNA probe molecule, this is almost
50°C below the Tm! It should not be surprising that
hybridization under these conditions leads to high background and
cross-hybridization. This low-stringency temperature was thought
necessary because RNA probe degradation was incorrectly attributed
to high-stringency hybridizations (probe degradation was actually
due to ribonuclease contamination). The inclusion of nonhomologous
nucleic acid blocking agents such as total yeast RNA (total yeast
RNA is better that tRNA), also contributes to the reduction of
cross-hybridization, particularly to ribosomal RNAs.
Choice of Membrane
To obtain the best results (i.e., high signal-to-noise
ratio and low backgrounds), the use of positively charged nylon
membranes such as Ambion's BrightStar™-Plus Nylon Membranes
is recommended, especially when working with nonisotopic probes.
Nitrocellulose membranes are not recommended, as they cannot withstand
the stringent hybridization and wash conditions used with RNA probes,
they cannot be stripped for re-hybridization, and they are incompatible
with virtually all nonisotopic detection protocols, including Ambion's
BrightStar™ Nonisotopic Detection System. Nitrocellulose also
cannot be used with rapid, one-hour transfer protocols like the
one used in the NorthernMax Kit.
After transfer, the RNA can be immobilized by
UV crosslinking the wet membrane (120 millijoules/cm2)
or by baking at 80°C for 15 minutes (vacuum not required for
nylon).
Hybridization and Washing Conditions
RNA:RNA duplexes have a higher Tm and
binding affinity than do RNA:DNA duplexes. As a result, the hybridization
buffer and temperature need to be adjusted to ensure optimal hybridization
to target and minimal nonspecific hybridization of probe, particularly
to the ribosomal sequences. The hybridization solution should be
formamide-based in order to lower the Tm of the RNA:RNA
duplex to a reasonable temperature; for most RNA probes this will
be around 60° to 65°C. When preparing hybridization buffer,
use only reagents known to be RNase-free. Avoid the use of products
derived from animal sources, in particular BSA and "BLOTTO". Salt
conditions (SSC or SSPE) between 500 mM and 1 M and SDS between
0.1% and 10% have been observed to provide good results (4). Use
only deionized, molecular biology grade formamide. Nucleic acid
blocking agents must be RNase-free as well. We have found the addition
100 µg/ml total yeast RNA (total yeast RNA performs better
than tRNA) helpful in reducing background and cross-hybridization.
Ambion's ULTRAhyb Hybridization Solution has incorporated all of
these recommendations and has been rigorously tested for nuclease
activity.
To approximate the Tm for RNA:RNA
duplexes, use the following formula:
|
Tm(RNA:RNA) |
|
|
= 78°C |
|
+ 16.6 x log10( [Na+] / (1.0 + 0.7[Na+]) ) |
|
+ 0.7 x (% GC) |
|
- 0.35 x (% formamide) |
|
- 500 / (duplex length) |
|
- 1°C / (% mismatch) |
Hybridization is performed at 15° to 25°C
below the calculated Tm. This will usually be 10°C
to 20°C higher than for a randomly primed DNA probe used to
detect the same mRNA target.
The final, stringent wash is generally performed
at the hybridization temperature in 0.1X SSC / 0.1% SDS or its
equivalent.
Stripping Blots for Re-Hybridization
Membranes can be stripped only if they
have never been allowed to dry to completion after hybridization.
Traditional procedures involve either boiling or autoclaving
(wet cycle) for ten minutes in a solution of 0.1% SDS in DEPC-treated
water, then cooling to room temperature. The chief drawback to
using RNA probes is that they are difficult to strip due to their
inherent high thermodynamic stability when hybridized to RNA
targets. Another important drawback is that these stripping conditions
will damage the RNA bound to the membrane after 3-4 strippings.
The harsh stripping conditions recommended
above are only possible because of the extremely high retention
of the recommended positively charged nylon membrane. As a precaution,
we recommend probing first for the mRNA you expect to be least
abundant. In case the probe is not completely removed, any residual
signal should not yet appear during the shorter exposure times
needed for more abundant probes.
Ambion's Strip-EZ™ Technology, however,
renders harsh stripping protocols as described above obsolete.
These probe synthesis kits generate probes that incoporate a
modified nucleotide. Following hybridization and detection of
the probe, a chemical in the probe degradation buffer provided
in the kit cleaves the modified nucleotides. The resulting probe
fragments are removed in a mild wash. Unlike the harsh treatments
commonly used to remove DNA probes from blots, the StripAble™ probe
removal protocol does not cause irreversible damage to the blot
that results in loss of sensitivity when the blot is re-probed.
This permits the use of the same blot repeatedly, enhancing consistency
of data and preserving precious nucleic acid samples.
References
- Current Protocols in Molecular
Biology (1995) John Willey & Sons, Inc. Vol. 1, 3.8.3
- Melton, D. A., Krieg, P.A., Rebagliati,
M.R., Maniatis, T., Zinn, K., and
Green, M.R. (1984) Efficient in vitro synthesis of biologically active
RNA and RNA hybridization probes from plasmids containing a bacteriophage SP6
promoter. Nucleic Acids Research 12: 7035-7056.
- Srivastava, R.A.K., and Schonfeld.
(1991) Use of riboprobes for Northern blotting analysis. BioTechniques 11:
584-587.
- Twomey, T.A. and Krawetz, S.A. (1990)
Parameters affecting hybridization of nucleic acids onto nylon
or nitrocellulose membranes. BioTechniques 8:
478-481.
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