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Silver staining of nucleic acids. Applications in virus research and in diagnostic virology
Journal of Virological Methods, 7 (1983) 185-198
185
Elsevier
SILVER STAINING RESEARCH
J. LINDSAY
OF NUCLEIC
ACIDS.
AND IN DIAGNOSTIC
WHITTON,
FIONA
APPLICATIONS
IN VIRUS
VIROLOGY
HUNDLEY,
BARBARA
O’DONNELL
and ULRICH
DESSELBERGER* Institute of Virology, University of Glasgow. and MRC Virology Unit, Church Street. Glasgow Gl I5JR. U.K. (Accepted
21 June
The rapid visualise
1983)
and sensitive
double-stranded
method
of silver staining
(ds) and single-stranded
silver ions to nucleic acids in gels is stoichiometric staining
can be applied
silver staining
to problems
DNA
RNA
acids in polyacrylamide
and independent
in virus research
viral genome
of nucleic
(ss) molecules
of the GC content
and to the analysis
analysis
gels is used to
of both DNA and RNA. The binding
diagnostic
of clinical
of
of ds DNA. Silver virus isolates.
virology
INTRODUCTION
Silver staining of gels containing proteins (Merril et al., 1979; Oakley et al., 1980; Merril et al., 1981; Morrissey, 1981; Sammons et al., 1981; Dubrayand Bezard, 1982), lipopolysaccharides (Tsai and Frasch, 1982) or nucleic acids (Somerville and Wang, 1981; Berry and Samuel, 1982; Herring et al., 1982; Follett and Desselberger, 1983) has recently been used in increasing frequency because the procedure is rapid and very sensitive. The present paper shows wider application of silver staining to nucleic acid analysis
in basic and diagnostic
virology.
Double-stranded
(ds) and single-stranded
(ss) molecules of both RNA and DNA. extracted from viruses and electrophoresed on polyacrylamide gels can be visualised to a similar degree of sensitivity. Evidence on the stoichiometry MATERIALS
of silver binding
to nucleic
acids is presented.
AND METHODS
Materials
Acrylamide, N,N’-methylenebisacrylamide and N,N,N,N’,-tetramethylethylenediamine were purchased from Bio-Rad; ultrapure urea was from Schwartz-Mann
*To whom correspondence
016609.34/83/$03.00
should
be addressed
0 1983 Elsevier Science Publishers
B.V.
and
186
ethidium bromide reagent grade. Preparation
was from
BDH
Chemicals.
All other
chemicals
used were of
of nucleic acids
ssRNAs
Human influenza viruses of types A and B were grown in embryonated eggs or on MDCK (canine kidney) cells, purified by ultracentrifugation through sucrose gradients (or through 30% sucrose cushions) and the RNA extracted as described previously (Palese and Schulman, 1976). The maximum amount from virus of one egg was approximately 1 pg. Virus harvested yielded less RNA which was not quantitated.
of RNA obtained per one Petri dish
dsRNAs
Rotavirus RNAs were prepared directly from human isolates (Follett and Desselberger, 1983). In most cases less than 1 pg of RNA was analysed; O.D. measurements of RNA extracts from human isolates were too low to allow accurate quantitation. ssDNAs 0X174
virion
ssDNA
was purchased
from New England
Biolabs.
dsDNAs
Herpes simplex virus type 1 (HSV-1 strain 17) and type 2 (HSV-2 strain HG52) and HSV isolates from patients were grown on confluent BHK 21 Cl3 cells and the DNA extracted from the supernatant of infected cultures (Hirt, 1967). The patients’isolates were passaged 2-4 times before use and titres of 10’ to lo* PFUs/ml DNA equivalent to 3 X 10’ to 3 X lo* PFUs of virus was analysed. quantitated after extraction. BamHI
fragments
of highly purified
HSV-2 (strain
were obtained. DNA was not
HG52) DNA were cloned into
the BamHI site of pAT153 and propagated in Escherichia coli K12 strain HBlOl as described (Davison and Wilkie, 1981). Adenoviruses were grown on 293 cells (Takiff et al., 1981) in single wells (20 mm diameter) of Linbro plates and the DNA extracted as described by Wade11 and de Jong (1980). A maximum of lo8 TCID,, of virus/Linbro well was obtained. No quantitation of extracted DNA was carried out. Fragments generated by Hae III digestion of oX174RF DNA were purchased from New England Biolabs. Restriction
endonucleases
Restriction endonucleases were purchased from Bethesda and used as described (Maniatis et al., 1982).
Research
Laboratories
187
Gel electrophoresis Electrophoresis of rotavirus and of influenza virus RNAs was carried out on 2.8% polyacrylamide 6 M urea slab gels (25 X 15 X 0.15 cm) using Loening’s buffer system (Palese and Schulman, 1976) at 150 V and 50-60 mA overnight. The same gel system was used to separate restriction endonuclease fragments of HSV DNAs and of adenovirus DNAs, and to electrophorese 0x174 virion DNA. The oX174RF DNA fragments and digests of cloned HSV-2 DNA fragments were subjected to electrophoresis at 70 V and 10 mA overnight on 5% polyacrylamide slab gels (25 X 15 X 0.15 cm) using ‘Tris-borate-EDTA (TBE) buffer (Maniatis et al., 1982). Silver staining Gels were stained
with silver nitrate
(pH 5) as originally
described
by Sammons
et
al. (1981) and as applied by Follett and Desselberger (1983). The only modification was termination of the reducing step by soaking the gels in 5% acetic acid (Herring et al., 1982). Gels were photographed using transmitted light and Ilford FP4 film. Ethidium
bromide staining
Gels were stained
in ethidium
bromide
(4 ug/ml)
in 1 X TBE.
Densitometry Ilford FP4 negatives were printed onto transparent bands measured using a Joyce Loebl Microdensitometer were calculated
by cutting
out peaks from photocopies
weighing them; the weights were converted the photocopy paper as reference. RESULTS
AND
film and the absorption of 3CS. The areas under peaks of densitometer
tracings
and
into areas using the weight of 100 mm2 of
DISCUSSION
dsRNAs Silver staining of the dsRNA segments of rotaviruses has recently been used to monitor the emergence of new strains in the human population (Follett and Desselberger, 1983) during outbreaks of infantile gastroenteritis and also to analyse rotaviruses isolated from calves (Herring et al., 1982). The sensitivity of silver staining of rotavirus RNA was found to be 0.3 to 0.4ng/segment (Herringet al., 1982). Similarly, subnanogram amounts of reovirus genomic dsRNA have been detected in polyacrylamide gels by silver staining (Berry and Samuel, 1982). In order to study quantitative aspects of silver ion binding to nucleic acids (Jensen
188
Fig. 1. Panel A: RNA of three independent separated
on a 2.8% polyacrylamide
described
in Materials
pattern
and methods.
Print made on transparent
2; that in lane 3 is of RNA pattern
gel indicate A. Numbers
the genomic under
segments.
peaks indicate
isolates of human
rotavirus
6 M urea slab gel. RNA preparation,
RNA segments.
and Desselberger,
electrophoresis
1983),
and staining
as
film. The RNAs in lanes 1 and 2are of RNA
1 (Follett and Desselberger.
Panel B: Densitometer
(Follett
1983). The numbers
curves of lanes 1-3 (indicated
to the right of the to the left)of panel
189
and Davidson, rotavirus transparent
RNA
1966) in polyacrylamide were silver stained
gels, gels containing and photographed.
film (Fig. IA) and densitometricaliy
evaluated
the separated Prints
segments
of
were then made on
(Fig. IB). Plots of the areas
under peaks of a densitometer tracing against the molecular weights of the RNA segments (Espejo et al., 1980) gave straight lines (Fig. 2) indicating a stoichiometric reaction of the rotavirus RNA with silver ions. This assumes that the RNA segments occur in equimolar amounts in the rotavirus virion as they do in reovirus particles (Shatkin et al., 1968). The fact that the straight lines of plots in Fig. 2 (and in Fig. 4B and 58, see below} cannot be extrapolated through zero is ascribed to background staining which occurred to variable degrees and increased with the amount of nucleic acid applied to a slot. When individual slots (width 5 mm) were loaded with more than 1 ug of rotavirus RNA (bovine rotavirus), the densitometry of each silver-stained segment gave a uniform maximum peak, showing that even the low molecular weight segments bound silver to an extent indistinguishable by densitometric analysis from that of the high molecular weight bands (unpubl. results).
moletulllr
might
(dalton.)
Fig. 2. Piot of areas under against the molecular (o), and lane 3 (0)
peaks of densitometer
weight (daltons)
ofsegments
tracings of rotavirus
(Fig. 18) of human
rotavirus
RNA. Values obtained
RNAs (Fig. 1A)
from lane
I (a),lane 2
P
191
ssRN.4~ Figure 3 shows the characteristic migration patterns on a polyacrylamide RNAs extracted from three influenza A and three influenza B virus strains.
gel of the Each track
was loaded with the RNA extracted from virus obtained from one infected egg (a maximum of 1 ug of RNA; tracks l-6) or from one 50 mm dish of infected MDCK cells (tracks 7-12). By using recent reference strains as standards, the procedure seems to be well suited to the rapid monitoring of both major and minor changes in the RNA migration patterns of new influenza virus isolates. A minimum of approximately 2 ng/RNA segment of influenza virus could be detected (results not shown), i.e. the procedure is slightly less sensitive than for dsRNAs (see above). When influenza virus RNA which had been labelled with 32P in infected MDCK cells (Palese and Schulman, 1976) was silver stained after separation on a polyacrylamide gel and then autoradiographed for several days, it was found that autoradiography was about ten times more sensitive than silver staining (results not shown). Silver staining has been successfully applied to monitor large scale purification of viroid RNA (D. Riesner, pers. comm.), a single-stranded covalently closed circular RNA with a high degree of internal base-pairing. ssDNi4s Samples containing different amounts of 0X174 ssDNA were run on a polyacrylamide gel and silver stained. A single band was found. The lowest detectable amount was approximately
2 ng (results
not shown).
dsDN.4s of dsDNA
Two sets of serial dilutions HaelII) were electrophoresed
Fig. 3. RNA from influenza slab gel. RNA preparation, was prepared
(oX174RF
type A and type B viruses was separated electrophoresis
from harvests
fragments
on the same 5% polyacrylamide
and staining
as described
DNA digested
with
gel. One group
was
on a 2.8% polyacrylamide under Materials
before virus inoculation,
1and 7, RNA of influenza virus A/PR/8/34 (H3N2); lanes 3 and 9, RNA ofinfluenza of Virology, influenza
Glasgow);
virus B/Hong
lanes 4 and 10, RNA of influenza Kong/8/73;
lanes 6and
changed
B/Maryland/57
in later isolates
strain
4 and
virus B/Maryland/57; of influenza
10). Migration
(lanes 2,3,8.9 and 5,6,11 and
vit’us A/Texas/l/77
(H3N2) (isolate 2974, January
12, RNA ofinfluenza
RNA segments
(lanes
to
seeded with 2 X IO6
lanes 7-12) was applied to each slot ofthe gel. Lanes
(H IN 1); lanes 2 and 8, RNA of influenza
virus A/Glasgow/82
to the right of lanes 1,4,7 and 10 indicate of influenza
RNA
of three eggs or three Petri dishes of MDCK cells and the RNA equivalent
virus grown in one egg (lanes 1-6) or in MDCK cells of one Petri dish (50 mm diameter, cells and grown to confluency
6 M urea
and methods.
12).
virus B/England/4/82. A/PR/8/34
1982, Institute
lanes 5 and
I I, RNA of The numbers
strain (lanes 1 and 7) and
of corresponding
RNA segments
has
12
3
6
5
4
7
8
9
lo
1353 1078 872
B area
under
wak
(mm’)
t 2oo
1
I
I
I
I
I
I
,
,
I
1
2
3
4
5
6
7
6
Q
b 10
molecular
mi6ht
(dalton8)
I 10-S
193
silver stained
and the other stained with ethidium
that bands representing detected ethidium
approximately
bromide,
The result (Fig, 4A)shows
0.5 ng of DNA (closed circles in Fig. 4A) were
by silver staining whereas the minimum amount of DNA detected by bromide staining was approximately 5 ng (open circles Fig. 4A). Therefore,
the sensitivity of silver staining of dsDNA was approximately ten times greater than that of ethidium bromide staining. The silver stained gel was subjected to densitometric analysis and Fig. 4B shows plots of areas under DNA peaks against their molecular weights. The straight lines obtained confirm the stoichiometric natureofthe reaction between silver ions and dsDNA. Jensen and Davidson (1966) had found that the strength of binding of silver ions to DNA in solution increased with increasing GC content at pH 5.6. It was of interest to establish whether or not this observation applied to the silver staining of DNA in gels. Hence, a dsDNA of known sequence (IL. Whitton et al., in prep.) was digested, yielding fragments of widely differing GC content. Figure 5A shows the silver stained gel and densitometric tracing of an AvaI digest of pBz (the BamHI z fragment of HSV-2 (strain HG52) cloned into pAT153). Figure 5B illustrates stoichiometric binding of silver ions by these DNA fragments in spite of the wide variation in GC content. The difference between this result and that of Jensen and Davidson (1966) may be due to the fact that the concentration of silver ions used to stain nucleic acids in gels is at least IOO~fold greater than that at which the differential effect of GC content on silver ion binding in solution was observed. Potential applications of silver staining to nucleic acid analysis in molecular biology are widespread. It allows the construction of detailed restriction maps of DNA fragments using ten-fold less DNA and restriction enzyme than DNA staining with ethidium bromide requires (L. Whitton, in prep.). Silver staining avoids two disadvantages associated with the use of nick-translated DNA for mapping purposes. Firstly, nick-translated
DNA
must be labelled
uniformly
and remain
sufficiently
intact
to
yield defined fragments after digestion. Secondly, nick-translated DNA fragments cannot be analysed on denaturing gels and therefore may not be sized accurately. Furthermore silver staining can be used to detect DNA:RNA hybrids such as those generated
by nuclease
ping (L. Whitton,
Fig. 4. Panel A: oX174RF silver stained; were: Tracks
DNA digested
tracks 6-10 stained
separated
bromide.
tracings
the number
gel. Tracks
1-5
of DNA applied to each track
3 and 8.40 ng; tracks 4 and 9, 20 ng; tracks 5 and fragment
in each track isindicated (not shown) against
of base pairs in each fragment
I (a), lane 2 (o), and lane 3 (0).
map-
outweighs
as deduced
from the DNA
to theleft ofeach bromidestained
the molecular
track by gel. Panel
weight (daltons)
for lanes I, 2 and 3 of the silver stained gel in Panel A. The molecular
by multiplying from lane
on a 5% polyacrylamide
gel and by open circles (0) on the ethidium
B: Plot of areas under peaks of densitometer
mRNA
of silver staining
The total amounts
on the left show the length in base pairs ofeach
(Sanger et al., 1978). The limit of detectability
the DNA fragments obtained
with IIaeIII,
with ethidium
closed circles (0) on the silver stained
calculated
1977), and hence facilitate
1 and 6, 160 ng; tracks 2 and 7, 80 ng; tracks
IO, 10 ng. The numbers sequence
Sl (Berk and Sharp,
in prep.). The high degree of sensitivity
(Panel A) by the factor
of
weights were 660. Values
194
A
1
L
18.1
9.1
4.4
3.2
23
1.3
1.1
0.99
54
63
80
72
73
63
67
60
mol~~lar (dsltonr)
wel9ht x IO-5
percentage GC content
2
4
6
8
10
12
14
16
18
20
molecutar wat9llt fdaltonr) x m-5
195
the fact that the staining bromide.
Silver staining
procedure
takes slightly
longer than staining
with ~thidium
of nucleic acids in gels is not suitable for preparative
purposes
as silver-stained nucleic acids cannot be eluted from gel slices (unpubl. results). Genomic analyses of clinical DNA virus isolates can be quickly performed using the silver staining procedure. HSV isolates from patients (identified as such by reacting reference HSV antisera with infected cells in an indirect immunofluorescence test) together with a reference strain of HSV 1 (strain 17) and a reference strain of HSV 2 (strain HG52) were grown and the DNAs extracted. Aliquots of DNA were then digested with different restriction enzymes and the fragments separated on polyacrylamide gels and silver stained. A representative result is shown in Fig. 6. All the clinical isolates were HSV-l and showed characteristic individual patterns deviating from that of the HSV-I reference strain and from each other (Lonsdale, 1979; Buchman et al., 1980). Adenovirus replicated in 293 cells of one Linbro plate well yielded enough DNA to be analysed in a silver stained polyacrylamide gel. Bgl II digests of adenovirus reference strains (of serotypes 2,5 and 7) are shownin Fig. 7. Digests of Hirt extracts (Wade11 and de Jong, 1980) from infected cells were compared with digests of DNA obtained from gradient-purified virions. The method is currently being used to investigate the genomes of clinical adenovirus isolates obtained during a local outbreak of keratoconjunctivitis (B. O’Donnell, unpubl. results). ACKNOWLEDGEMENTS
We thank Dr. Andrew Davison for discussion and for initially supplying us with a BamHI digest of DNA from purified HSV-1 and HSV-2, Dr. Vivien Mautner for advice and for providing us with DNA from purified adenovirus of different serotypes, and Dr. J. Barklie Clements JLW was supported by a Medical
for critical reading of the manuscript. Research Council Training Fellowship
Fig. 5 Panel A: The lower part shows a lane of a 5% polyacrylamide have been separated
fragments
cloned into the BarnHI
fragmsent are shown. The densitometer peaks
of densitometer
calculated
by multiplying
tracing
gel (run from left to right) on which
from an Ava I digest of pBz (the BamHI z fragment
site of pAT153).
The molecular tracing
in Fig. 5A against
the number
weight (daltons)
is displayed
G84/785.
of HSV 2 (strain HG52)
and the GC content
(%) of each
above the gel lane. Panel B: Plot of areas under
the molecular
of base pairs in each fragment
weights
(daltons)
(Whitton
of the fragments,
et al.. in prep.)
by 660.
196
A 1
E3 1
23456789
Fig. 6. BamHI
digests of HSV DNA separated
and silver staining
as described
Tracks
1-7, independently
(strain
17) reference
1, HSV 2 (strain experiments.
strains. HG52);
in Materials
obtained
on a 2.8% polyacrylamide
and methods.
6 M urea slab gel. Electrophoresis
Panel A: Hirt extracts (Hirt, 1967) of HSV DNA.
clinical HSV isolates; track 8, HSV 2 (strain HG52), and track 9. HSV I
Panel B: HSV reference track
2
2. HSV
I (strain
strains purified
and extracted
17). The gels in panels
as described
(16). Track
A and B are from different
197
Fig. 7. Hgl II digests of adenovirus
DNAs of serotypes
2 (lanes 5 and 6), 5 (lanes 3 and 4) and 7 (lanes
1and
2). DNA extracts
from infected cells (Wade11 and de Jon& 1980; lanes I, 3 and 5) and from purified virions 6 M urea siab gel. (lanes 2, 4 and 6: 0.2 pip of DNA was used) were separated on a 2.8% polyacrytamide Electrophoresis represent
residual
and silver staining partially
digested
as described
in Materials
DNA fragments.
and methods.
The faint bands
in track
6
198
REFERENCES
Berk, A.J. and P.A. Sharp,
1977, Cell 12, 721-732.
Berry, M.J. and C.E. Samuel, Buchman,
T.G., T. Simpson,
1982, Anal. Biochem. C. Nosal, B. Roizman
124, 180-184. and A. Nahmias,
1980, Ann. N.Y. Acad. Sci. 354,279-
290. Davison,
A.J. and N.M. Wilkie,
Dubray,
G. and G. Bezard,
Espejo,
R., E. Martinez,
Follett,
E.A.C.
Herring,
1981, J. Gen. Viral. 5.5, 315-331.
1982, Anal. Biochem.
S. Lopez and 0. Mutioz,
and U. Desselberger.
119, 325-329. 1980, Inf. Immunol.
1983, J. Med. Viral.
A.J.. N. Inglis, C.K. Ojeh, D.R. Snodgrass
28, 230-237.
11, 39-52.
and J.D. Menzies,
1982, J. Clin. Microbial.
16,473-
477. Hirt, B. (1967) J. Mol. Biol. 26, 365-369. Jensen,
R.H. and N. Davidson,
Lonsdale,
D.M.,
Maniatis, Spring
T., E.F. Fritsch and J. Sambrook,
1982, Molecular Harbor.
Laboratory,
C.R., R.C. Schwitzer
Merril,
C.R., D. Goldman,
Morrissey,
J.H.,
Cold Spring
and H.L. van Keuren, S.A. Sedman
1981, Anal.
B.R., D.R. Kirsch
Biochem.
and E.E. Nishizawa,
P.M. Slocombe Shatkin,
T. Friedman,
and M. Smith,
L.L. and K. Wang,
H.E., S.E. Straus
Wadell,
Sci. U.S.A.
G. and J.C. de Jong,
p, 104. Cold
76, 4335-4339.
Biochem.
105, 361-363.
17, 876-884. 1981, Electrophoresis
G.N. Air, B.G. Barrell,
2, 135-141.
N.L. Brown,
J.C. Fiddes,
1978, J. Mol. Biol. 125, 225-246. 1981, Biochem.
and C.F. Garon,
Tsai, C.M. and C.E. Frasch,
Manual,
1981, Science 211, 1437-1438.
A.J., J.D. Sipe and P.C. Loh, 1968, J. Viral. 2, 986-991.
Somerville, Takiff,
L.D. Adams
1979, Proc. Natl. Acad.
1980, Anal.
Sammons,
D.W.,
A Laboratory
117, 307-310.
and N.R. Morris, 1976, J. Viral.
F., R. Coulson,
Cloning.
and M.H. Ebert,
Palese, P. and J.L. Schulman, Sanger,
4, 17-32.
I, 849-852.
Harbor
Merril,
Oakley,
1966, Biopolymers
1979, Lancet
1982, Anal.
Biophys.
1981, Lancet Biochem.
1980, Inf. Immunol.
Res. Comm. II, 832-834.
119, 115-l 19. 27, 292-296.
102, 53-58.
C.A. Hutchison,
185
Elsevier
SILVER STAINING RESEARCH
J. LINDSAY
OF NUCLEIC
ACIDS.
AND IN DIAGNOSTIC
WHITTON,
FIONA
APPLICATIONS
IN VIRUS
VIROLOGY
HUNDLEY,
BARBARA
O’DONNELL
and ULRICH
DESSELBERGER* Institute of Virology, University of Glasgow. and MRC Virology Unit, Church Street. Glasgow Gl I5JR. U.K. (Accepted
21 June
The rapid visualise
1983)
and sensitive
double-stranded
method
of silver staining
(ds) and single-stranded
silver ions to nucleic acids in gels is stoichiometric staining
can be applied
silver staining
to problems
DNA
RNA
acids in polyacrylamide
and independent
in virus research
viral genome
of nucleic
(ss) molecules
of the GC content
and to the analysis
analysis
gels is used to
of both DNA and RNA. The binding
diagnostic
of clinical
of
of ds DNA. Silver virus isolates.
virology
INTRODUCTION
Silver staining of gels containing proteins (Merril et al., 1979; Oakley et al., 1980; Merril et al., 1981; Morrissey, 1981; Sammons et al., 1981; Dubrayand Bezard, 1982), lipopolysaccharides (Tsai and Frasch, 1982) or nucleic acids (Somerville and Wang, 1981; Berry and Samuel, 1982; Herring et al., 1982; Follett and Desselberger, 1983) has recently been used in increasing frequency because the procedure is rapid and very sensitive. The present paper shows wider application of silver staining to nucleic acid analysis
in basic and diagnostic
virology.
Double-stranded
(ds) and single-stranded
(ss) molecules of both RNA and DNA. extracted from viruses and electrophoresed on polyacrylamide gels can be visualised to a similar degree of sensitivity. Evidence on the stoichiometry MATERIALS
of silver binding
to nucleic
acids is presented.
AND METHODS
Materials
Acrylamide, N,N’-methylenebisacrylamide and N,N,N,N’,-tetramethylethylenediamine were purchased from Bio-Rad; ultrapure urea was from Schwartz-Mann
*To whom correspondence
016609.34/83/$03.00
should
be addressed
0 1983 Elsevier Science Publishers
B.V.
and
186
ethidium bromide reagent grade. Preparation
was from
BDH
Chemicals.
All other
chemicals
used were of
of nucleic acids
ssRNAs
Human influenza viruses of types A and B were grown in embryonated eggs or on MDCK (canine kidney) cells, purified by ultracentrifugation through sucrose gradients (or through 30% sucrose cushions) and the RNA extracted as described previously (Palese and Schulman, 1976). The maximum amount from virus of one egg was approximately 1 pg. Virus harvested yielded less RNA which was not quantitated.
of RNA obtained per one Petri dish
dsRNAs
Rotavirus RNAs were prepared directly from human isolates (Follett and Desselberger, 1983). In most cases less than 1 pg of RNA was analysed; O.D. measurements of RNA extracts from human isolates were too low to allow accurate quantitation. ssDNAs 0X174
virion
ssDNA
was purchased
from New England
Biolabs.
dsDNAs
Herpes simplex virus type 1 (HSV-1 strain 17) and type 2 (HSV-2 strain HG52) and HSV isolates from patients were grown on confluent BHK 21 Cl3 cells and the DNA extracted from the supernatant of infected cultures (Hirt, 1967). The patients’isolates were passaged 2-4 times before use and titres of 10’ to lo* PFUs/ml DNA equivalent to 3 X 10’ to 3 X lo* PFUs of virus was analysed. quantitated after extraction. BamHI
fragments
of highly purified
HSV-2 (strain
were obtained. DNA was not
HG52) DNA were cloned into
the BamHI site of pAT153 and propagated in Escherichia coli K12 strain HBlOl as described (Davison and Wilkie, 1981). Adenoviruses were grown on 293 cells (Takiff et al., 1981) in single wells (20 mm diameter) of Linbro plates and the DNA extracted as described by Wade11 and de Jong (1980). A maximum of lo8 TCID,, of virus/Linbro well was obtained. No quantitation of extracted DNA was carried out. Fragments generated by Hae III digestion of oX174RF DNA were purchased from New England Biolabs. Restriction
endonucleases
Restriction endonucleases were purchased from Bethesda and used as described (Maniatis et al., 1982).
Research
Laboratories
187
Gel electrophoresis Electrophoresis of rotavirus and of influenza virus RNAs was carried out on 2.8% polyacrylamide 6 M urea slab gels (25 X 15 X 0.15 cm) using Loening’s buffer system (Palese and Schulman, 1976) at 150 V and 50-60 mA overnight. The same gel system was used to separate restriction endonuclease fragments of HSV DNAs and of adenovirus DNAs, and to electrophorese 0x174 virion DNA. The oX174RF DNA fragments and digests of cloned HSV-2 DNA fragments were subjected to electrophoresis at 70 V and 10 mA overnight on 5% polyacrylamide slab gels (25 X 15 X 0.15 cm) using ‘Tris-borate-EDTA (TBE) buffer (Maniatis et al., 1982). Silver staining Gels were stained
with silver nitrate
(pH 5) as originally
described
by Sammons
et
al. (1981) and as applied by Follett and Desselberger (1983). The only modification was termination of the reducing step by soaking the gels in 5% acetic acid (Herring et al., 1982). Gels were photographed using transmitted light and Ilford FP4 film. Ethidium
bromide staining
Gels were stained
in ethidium
bromide
(4 ug/ml)
in 1 X TBE.
Densitometry Ilford FP4 negatives were printed onto transparent bands measured using a Joyce Loebl Microdensitometer were calculated
by cutting
out peaks from photocopies
weighing them; the weights were converted the photocopy paper as reference. RESULTS
AND
film and the absorption of 3CS. The areas under peaks of densitometer
tracings
and
into areas using the weight of 100 mm2 of
DISCUSSION
dsRNAs Silver staining of the dsRNA segments of rotaviruses has recently been used to monitor the emergence of new strains in the human population (Follett and Desselberger, 1983) during outbreaks of infantile gastroenteritis and also to analyse rotaviruses isolated from calves (Herring et al., 1982). The sensitivity of silver staining of rotavirus RNA was found to be 0.3 to 0.4ng/segment (Herringet al., 1982). Similarly, subnanogram amounts of reovirus genomic dsRNA have been detected in polyacrylamide gels by silver staining (Berry and Samuel, 1982). In order to study quantitative aspects of silver ion binding to nucleic acids (Jensen
188
Fig. 1. Panel A: RNA of three independent separated
on a 2.8% polyacrylamide
described
in Materials
pattern
and methods.
Print made on transparent
2; that in lane 3 is of RNA pattern
gel indicate A. Numbers
the genomic under
segments.
peaks indicate
isolates of human
rotavirus
6 M urea slab gel. RNA preparation,
RNA segments.
and Desselberger,
electrophoresis
1983),
and staining
as
film. The RNAs in lanes 1 and 2are of RNA
1 (Follett and Desselberger.
Panel B: Densitometer
(Follett
1983). The numbers
curves of lanes 1-3 (indicated
to the right of the to the left)of panel
189
and Davidson, rotavirus transparent
RNA
1966) in polyacrylamide were silver stained
gels, gels containing and photographed.
film (Fig. IA) and densitometricaliy
evaluated
the separated Prints
segments
of
were then made on
(Fig. IB). Plots of the areas
under peaks of a densitometer tracing against the molecular weights of the RNA segments (Espejo et al., 1980) gave straight lines (Fig. 2) indicating a stoichiometric reaction of the rotavirus RNA with silver ions. This assumes that the RNA segments occur in equimolar amounts in the rotavirus virion as they do in reovirus particles (Shatkin et al., 1968). The fact that the straight lines of plots in Fig. 2 (and in Fig. 4B and 58, see below} cannot be extrapolated through zero is ascribed to background staining which occurred to variable degrees and increased with the amount of nucleic acid applied to a slot. When individual slots (width 5 mm) were loaded with more than 1 ug of rotavirus RNA (bovine rotavirus), the densitometry of each silver-stained segment gave a uniform maximum peak, showing that even the low molecular weight segments bound silver to an extent indistinguishable by densitometric analysis from that of the high molecular weight bands (unpubl. results).
moletulllr
might
(dalton.)
Fig. 2. Piot of areas under against the molecular (o), and lane 3 (0)
peaks of densitometer
weight (daltons)
ofsegments
tracings of rotavirus
(Fig. 18) of human
rotavirus
RNA. Values obtained
RNAs (Fig. 1A)
from lane
I (a),lane 2
P
191
ssRN.4~ Figure 3 shows the characteristic migration patterns on a polyacrylamide RNAs extracted from three influenza A and three influenza B virus strains.
gel of the Each track
was loaded with the RNA extracted from virus obtained from one infected egg (a maximum of 1 ug of RNA; tracks l-6) or from one 50 mm dish of infected MDCK cells (tracks 7-12). By using recent reference strains as standards, the procedure seems to be well suited to the rapid monitoring of both major and minor changes in the RNA migration patterns of new influenza virus isolates. A minimum of approximately 2 ng/RNA segment of influenza virus could be detected (results not shown), i.e. the procedure is slightly less sensitive than for dsRNAs (see above). When influenza virus RNA which had been labelled with 32P in infected MDCK cells (Palese and Schulman, 1976) was silver stained after separation on a polyacrylamide gel and then autoradiographed for several days, it was found that autoradiography was about ten times more sensitive than silver staining (results not shown). Silver staining has been successfully applied to monitor large scale purification of viroid RNA (D. Riesner, pers. comm.), a single-stranded covalently closed circular RNA with a high degree of internal base-pairing. ssDNi4s Samples containing different amounts of 0X174 ssDNA were run on a polyacrylamide gel and silver stained. A single band was found. The lowest detectable amount was approximately
2 ng (results
not shown).
dsDN.4s of dsDNA
Two sets of serial dilutions HaelII) were electrophoresed
Fig. 3. RNA from influenza slab gel. RNA preparation, was prepared
(oX174RF
type A and type B viruses was separated electrophoresis
from harvests
fragments
on the same 5% polyacrylamide
and staining
as described
DNA digested
with
gel. One group
was
on a 2.8% polyacrylamide under Materials
before virus inoculation,
1and 7, RNA of influenza virus A/PR/8/34 (H3N2); lanes 3 and 9, RNA ofinfluenza of Virology, influenza
Glasgow);
virus B/Hong
lanes 4 and 10, RNA of influenza Kong/8/73;
lanes 6and
changed
B/Maryland/57
in later isolates
strain
4 and
virus B/Maryland/57; of influenza
10). Migration
(lanes 2,3,8.9 and 5,6,11 and
vit’us A/Texas/l/77
(H3N2) (isolate 2974, January
12, RNA ofinfluenza
RNA segments
(lanes
to
seeded with 2 X IO6
lanes 7-12) was applied to each slot ofthe gel. Lanes
(H IN 1); lanes 2 and 8, RNA of influenza
virus A/Glasgow/82
to the right of lanes 1,4,7 and 10 indicate of influenza
RNA
of three eggs or three Petri dishes of MDCK cells and the RNA equivalent
virus grown in one egg (lanes 1-6) or in MDCK cells of one Petri dish (50 mm diameter, cells and grown to confluency
6 M urea
and methods.
12).
virus B/England/4/82. A/PR/8/34
1982, Institute
lanes 5 and
I I, RNA of The numbers
strain (lanes 1 and 7) and
of corresponding
RNA segments
has
12
3
6
5
4
7
8
9
lo
1353 1078 872
B area
under
wak
(mm’)
t 2oo
1
I
I
I
I
I
I
,
,
I
1
2
3
4
5
6
7
6
Q
b 10
molecular
mi6ht
(dalton8)
I 10-S
193
silver stained
and the other stained with ethidium
that bands representing detected ethidium
approximately
bromide,
The result (Fig, 4A)shows
0.5 ng of DNA (closed circles in Fig. 4A) were
by silver staining whereas the minimum amount of DNA detected by bromide staining was approximately 5 ng (open circles Fig. 4A). Therefore,
the sensitivity of silver staining of dsDNA was approximately ten times greater than that of ethidium bromide staining. The silver stained gel was subjected to densitometric analysis and Fig. 4B shows plots of areas under DNA peaks against their molecular weights. The straight lines obtained confirm the stoichiometric natureofthe reaction between silver ions and dsDNA. Jensen and Davidson (1966) had found that the strength of binding of silver ions to DNA in solution increased with increasing GC content at pH 5.6. It was of interest to establish whether or not this observation applied to the silver staining of DNA in gels. Hence, a dsDNA of known sequence (IL. Whitton et al., in prep.) was digested, yielding fragments of widely differing GC content. Figure 5A shows the silver stained gel and densitometric tracing of an AvaI digest of pBz (the BamHI z fragment of HSV-2 (strain HG52) cloned into pAT153). Figure 5B illustrates stoichiometric binding of silver ions by these DNA fragments in spite of the wide variation in GC content. The difference between this result and that of Jensen and Davidson (1966) may be due to the fact that the concentration of silver ions used to stain nucleic acids in gels is at least IOO~fold greater than that at which the differential effect of GC content on silver ion binding in solution was observed. Potential applications of silver staining to nucleic acid analysis in molecular biology are widespread. It allows the construction of detailed restriction maps of DNA fragments using ten-fold less DNA and restriction enzyme than DNA staining with ethidium bromide requires (L. Whitton, in prep.). Silver staining avoids two disadvantages associated with the use of nick-translated DNA for mapping purposes. Firstly, nick-translated
DNA
must be labelled
uniformly
and remain
sufficiently
intact
to
yield defined fragments after digestion. Secondly, nick-translated DNA fragments cannot be analysed on denaturing gels and therefore may not be sized accurately. Furthermore silver staining can be used to detect DNA:RNA hybrids such as those generated
by nuclease
ping (L. Whitton,
Fig. 4. Panel A: oX174RF silver stained; were: Tracks
DNA digested
tracks 6-10 stained
separated
bromide.
tracings
the number
gel. Tracks
1-5
of DNA applied to each track
3 and 8.40 ng; tracks 4 and 9, 20 ng; tracks 5 and fragment
in each track isindicated (not shown) against
of base pairs in each fragment
I (a), lane 2 (o), and lane 3 (0).
map-
outweighs
as deduced
from the DNA
to theleft ofeach bromidestained
the molecular
track by gel. Panel
weight (daltons)
for lanes I, 2 and 3 of the silver stained gel in Panel A. The molecular
by multiplying from lane
on a 5% polyacrylamide
gel and by open circles (0) on the ethidium
B: Plot of areas under peaks of densitometer
mRNA
of silver staining
The total amounts
on the left show the length in base pairs ofeach
(Sanger et al., 1978). The limit of detectability
the DNA fragments obtained
with IIaeIII,
with ethidium
closed circles (0) on the silver stained
calculated
1977), and hence facilitate
1 and 6, 160 ng; tracks 2 and 7, 80 ng; tracks
IO, 10 ng. The numbers sequence
Sl (Berk and Sharp,
in prep.). The high degree of sensitivity
(Panel A) by the factor
of
weights were 660. Values
194
A
1
L
18.1
9.1
4.4
3.2
23
1.3
1.1
0.99
54
63
80
72
73
63
67
60
mol~~lar (dsltonr)
wel9ht x IO-5
percentage GC content
2
4
6
8
10
12
14
16
18
20
molecutar wat9llt fdaltonr) x m-5
195
the fact that the staining bromide.
Silver staining
procedure
takes slightly
longer than staining
with ~thidium
of nucleic acids in gels is not suitable for preparative
purposes
as silver-stained nucleic acids cannot be eluted from gel slices (unpubl. results). Genomic analyses of clinical DNA virus isolates can be quickly performed using the silver staining procedure. HSV isolates from patients (identified as such by reacting reference HSV antisera with infected cells in an indirect immunofluorescence test) together with a reference strain of HSV 1 (strain 17) and a reference strain of HSV 2 (strain HG52) were grown and the DNAs extracted. Aliquots of DNA were then digested with different restriction enzymes and the fragments separated on polyacrylamide gels and silver stained. A representative result is shown in Fig. 6. All the clinical isolates were HSV-l and showed characteristic individual patterns deviating from that of the HSV-I reference strain and from each other (Lonsdale, 1979; Buchman et al., 1980). Adenovirus replicated in 293 cells of one Linbro plate well yielded enough DNA to be analysed in a silver stained polyacrylamide gel. Bgl II digests of adenovirus reference strains (of serotypes 2,5 and 7) are shownin Fig. 7. Digests of Hirt extracts (Wade11 and de Jong, 1980) from infected cells were compared with digests of DNA obtained from gradient-purified virions. The method is currently being used to investigate the genomes of clinical adenovirus isolates obtained during a local outbreak of keratoconjunctivitis (B. O’Donnell, unpubl. results). ACKNOWLEDGEMENTS
We thank Dr. Andrew Davison for discussion and for initially supplying us with a BamHI digest of DNA from purified HSV-1 and HSV-2, Dr. Vivien Mautner for advice and for providing us with DNA from purified adenovirus of different serotypes, and Dr. J. Barklie Clements JLW was supported by a Medical
for critical reading of the manuscript. Research Council Training Fellowship
Fig. 5 Panel A: The lower part shows a lane of a 5% polyacrylamide have been separated
fragments
cloned into the BarnHI
fragmsent are shown. The densitometer peaks
of densitometer
calculated
by multiplying
tracing
gel (run from left to right) on which
from an Ava I digest of pBz (the BamHI z fragment
site of pAT153).
The molecular tracing
in Fig. 5A against
the number
weight (daltons)
is displayed
G84/785.
of HSV 2 (strain HG52)
and the GC content
(%) of each
above the gel lane. Panel B: Plot of areas under
the molecular
of base pairs in each fragment
weights
(daltons)
(Whitton
of the fragments,
et al.. in prep.)
by 660.
196
A 1
E3 1
23456789
Fig. 6. BamHI
digests of HSV DNA separated
and silver staining
as described
Tracks
1-7, independently
(strain
17) reference
1, HSV 2 (strain experiments.
strains. HG52);
in Materials
obtained
on a 2.8% polyacrylamide
and methods.
6 M urea slab gel. Electrophoresis
Panel A: Hirt extracts (Hirt, 1967) of HSV DNA.
clinical HSV isolates; track 8, HSV 2 (strain HG52), and track 9. HSV I
Panel B: HSV reference track
2
2. HSV
I (strain
strains purified
and extracted
17). The gels in panels
as described
(16). Track
A and B are from different
197
Fig. 7. Hgl II digests of adenovirus
DNAs of serotypes
2 (lanes 5 and 6), 5 (lanes 3 and 4) and 7 (lanes
1and
2). DNA extracts
from infected cells (Wade11 and de Jon& 1980; lanes I, 3 and 5) and from purified virions 6 M urea siab gel. (lanes 2, 4 and 6: 0.2 pip of DNA was used) were separated on a 2.8% polyacrytamide Electrophoresis represent
residual
and silver staining partially
digested
as described
in Materials
DNA fragments.
and methods.
The faint bands
in track
6
198
REFERENCES
Berk, A.J. and P.A. Sharp,
1977, Cell 12, 721-732.
Berry, M.J. and C.E. Samuel, Buchman,
T.G., T. Simpson,
1982, Anal. Biochem. C. Nosal, B. Roizman
124, 180-184. and A. Nahmias,
1980, Ann. N.Y. Acad. Sci. 354,279-
290. Davison,
A.J. and N.M. Wilkie,
Dubray,
G. and G. Bezard,
Espejo,
R., E. Martinez,
Follett,
E.A.C.
Herring,
1981, J. Gen. Viral. 5.5, 315-331.
1982, Anal. Biochem.
S. Lopez and 0. Mutioz,
and U. Desselberger.
119, 325-329. 1980, Inf. Immunol.
1983, J. Med. Viral.
A.J.. N. Inglis, C.K. Ojeh, D.R. Snodgrass
28, 230-237.
11, 39-52.
and J.D. Menzies,
1982, J. Clin. Microbial.
16,473-
477. Hirt, B. (1967) J. Mol. Biol. 26, 365-369. Jensen,
R.H. and N. Davidson,
Lonsdale,
D.M.,
Maniatis, Spring
T., E.F. Fritsch and J. Sambrook,
1982, Molecular Harbor.
Laboratory,
C.R., R.C. Schwitzer
Merril,
C.R., D. Goldman,
Morrissey,
J.H.,
Cold Spring
and H.L. van Keuren, S.A. Sedman
1981, Anal.
B.R., D.R. Kirsch
Biochem.
and E.E. Nishizawa,
P.M. Slocombe Shatkin,
T. Friedman,
and M. Smith,
L.L. and K. Wang,
H.E., S.E. Straus
Wadell,
Sci. U.S.A.
G. and J.C. de Jong,
p, 104. Cold
76, 4335-4339.
Biochem.
105, 361-363.
17, 876-884. 1981, Electrophoresis
G.N. Air, B.G. Barrell,
2, 135-141.
N.L. Brown,
J.C. Fiddes,
1978, J. Mol. Biol. 125, 225-246. 1981, Biochem.
and C.F. Garon,
Tsai, C.M. and C.E. Frasch,
Manual,
1981, Science 211, 1437-1438.
A.J., J.D. Sipe and P.C. Loh, 1968, J. Viral. 2, 986-991.
Somerville, Takiff,
L.D. Adams
1979, Proc. Natl. Acad.
1980, Anal.
Sammons,
D.W.,
A Laboratory
117, 307-310.
and N.R. Morris, 1976, J. Viral.
F., R. Coulson,
Cloning.
and M.H. Ebert,
Palese, P. and J.L. Schulman, Sanger,
4, 17-32.
I, 849-852.
Harbor
Merril,
Oakley,
1966, Biopolymers
1979, Lancet
1982, Anal.
Biophys.
1981, Lancet Biochem.
1980, Inf. Immunol.
Res. Comm. II, 832-834.
119, 115-l 19. 27, 292-296.
102, 53-58.
C.A. Hutchison,