Nucleic acid amplification is the core technology of molecular biology and genetic engineering. Various isothermal amplification techniques have been developed as alternatives to polymerase chain reaction (PCR). However, most of these methods can only detect single stranded nucleic acid. Herein, we put forward a simple solution for opening double-stranded DNA for isothermal detection methods. The strategy employs recombination protein from E. coli (RecA) to form nucleoprotein complex with single-stranded DNA, which could scan double-stranded template for homologous sites. Then, the nucleoprotein can invade the double-stranded template to form heteroduplex in the presence of ATP, resulting in the strand exchange. The ATP regeneration system could be eliminated by using high concentration of ATP, and the 3'-OH terminal of the invasion strand can be recognized by other DNA modifying enzymes such as DNA polymerase or DNA ligase. Moreover, dATP was found to be a better cofactor for RecA, which make the system more compatible to DNA polymerase. The method described here is a general solution to open dsDNA, serving as a platform to develop more isothermal nucleic acids detection methods for real DNA samples based on it.
Nucleic acid amplification is the core technology of molecular biology and genetic engineering. Various isothermal amplification techniques have been developed as alternatives to polymerase chain reaction (PCR). However, most of these methods can only detect single stranded nucleic acid. Herein, we put forward a simple solution for opening double-stranded DNA for isothermal detection methods. The strategy employs recombination protein from E. coli (RecA) to form nucleoprotein complex with single-stranded DNA, which could scan double-stranded template for homologous sites. Then, the nucleoprotein can invade the double-stranded template to form heteroduplex in the presence of ATP, resulting in the strand exchange. The ATP regeneration system could be eliminated by using high concentration of ATP, and the 3'-OH terminal of the invasion strand can be recognized by other DNA modifying enzymes such as DNA polymerase or DNA ligase. Moreover, dATP was found to be a better cofactor for RecA, which make the system more compatible to DNA polymerase. The method described here is a general solution to open dsDNA, serving as a platform to develop more isothermal nucleic acids detection methods for real DNA samples based on it.
Highly sensitive and selective DNA detection methods are important scientific tools in
molecular biology and medical research. Many analytical methods for specific nucleic
acid quantification have been developed1234567. Polymerase
chain reaction (PCR) is a widely used technology because of its remarkably high
rapidity, precision and reproducibility891011121314. Based on
the thermal cycling system (PCR machine), duplex DNA targets and amplicons could
be separated at denaturation temperature, yielding two single stranded DNA as templates
for next round of amplification. The following primer annealing and elongation on the
template will carry out at different temperatures. Therefore, sophisticated equipment
for precise temperature control and thermal stable DNA polymerase are indispensable for
this method, which has limited its application in unspecialized laboratory and on-site
tests. These limitations in PCR-based techniques have spurred the development of a new
molecular-biological technique known as isothermal DNA amplification15161718192021. As only a single optimal reaction temperature
is required for the entire detection, isothermal amplification could satisfy rapid
on-site detection of environmental, foodborne, and water-borne pathogens as well as for
point-of-care clinical diagnostics, providing simpler and more effective reaction
conditions without expensive equipment. So far, a lot of isothermal DNA amplification
technologies, including NASBA15, SDA16,
RCA18, HDA19, LAMP21 and so on ref. 22, have been developed as promising
alternatives of thermal cycling based technique. However, most of isothermal
amplification methods can only detect single-stranded nucleic acid. To apply those
methods in the detection of double-stranded DNA, extra steps to obtain the single
stranded DNA through heat denaturation are required. One solution to open double
stranded DNA is to preheat the DNA sample at 95 °C with two
pairs of primers before isothermal amplification (Fig. 1A). Then
the outer primers and inner primers are annealed to corresponding unwound single
stranded template which would be extended by DNA polymerase with strand displacement
activity to displace the elongated product of inner primers, yielding the
single-stranded DNA to initiate the following isothermal amplification. However, the
pre-denaturation step is dependent of heating equipment, making it impossible for these
methods to achieve in one step. Recently, a novel isothermal DNA amplification method
named recombinase polymerase amplification (RPA) has been reported20. Instead of using high temperature to achieve the denaturation of the double-stranded
DNA target, RPA utilize recombinase enzyme to form complex with ssDNA primer that
could search for DNA sequence homology on the double stranded DNA target, facilitating
the strand exchange between dsDNA and single stranded primer to form D-loop. Then the
primer can be extended by DNA polymerase with strand-displacement activity (Fig. 1B). Compared to other isothermal amplification methods like
HDA19 and LAMP21 that need preheating to
open dsDNA or constant high temperature for entire processes, RPA is the only
isothermal method that could work at 37 °C because of the
application of recombinase. To facilitate the DNA replication, two more proteins besides
recombinase uvsX are indispensable in RPA: uvsY for stabilizing
interactions between uvsX and ssDNA and gp32 for stabilization of the
displaced ssDNA (Fig. 1B), moreover, an ATP regeneration system
are required to supplement the ATP consumed in the process of DNA substitution. Three
proteins applied in RPA are unavailable commercially and all those enzymes are
obtained from T4 phage that was a considerable threat for widely used engineered
bacterium for large-scale preparation. As the critical component in RPA,
uvsX is the recombinase of T4 phage. Recombinase are ubiquitous proteins
found in almost all organisms, including RecA from bacteria, Rad51 and
Dmc1 from eukaryotes, and RadA from archaea. They are important
proteins participating in many biological processes such as double-strand DNA break
(DSB) repair, rescue of stalled or collapsed replication forks, chromosomal
rearrangements and horizontal gene transfer23. Up to now, RecA of
E. coli is the only commercial available recombinase and has been extensively
studied. And the substantial function of RecA
in vivo is to form nucleoprotein complex with transient single-stranded DNA and
facilitate strand exchange with homologous duplex24. Therefore, we ask
this question: Can we utilize the recombinaseRecA of E. coli as a tool to
open double-stranded DNA for isothermal detection methods. To achieve this goal, there
are three challenges we need to address: 1. Even it have been reported that RecA
can promote the formation of D-loop in the presence of ATP25, whether the
complex formed by RecA and short ssDNA can invade into duplex DNA to substitute
the identical strand? 2. It is known that RecA, as a single-stranded DNA
dependent ATPase, could bind with single-stranded DNA to hydrolyze ATP into ADP
immediately and dissociates from single-stranded DNA as a result. However, it is still
ambiguous and controversial whether hydrolysis of ATP is needed to realize DNA strand
exchange26272829. 3. Though RecA could open dsDNA target
with short ssDNA, it is not clear whether the 3′-OH terminal of the invasion
strand can be recognized by other DNA modifying enzymes such as DNA polymerase or DNA
ligase. Herein, we report the research to figure out these problems and establish a
general solution to open double-stranded DNA for the different isothermal detection
methods using RecA protein from E. coli.
Figure 1
(A) The strategy to open dsDNA to produce ssDNA for isothermal
detection methods. After the double-stranded DNA is denatured by heating,
two pairs of ssDNA primer could anneal to the corresponding single-stranded
DNA. Then the primers are extended by DNA polymerase with strand
displacement activity. The extension of the outer primers results in the
displacement of the elongated products of the inner primers, forming ssDNA.
(B) Dynamic processes in recombinase polymerase amplification
(RPA). In the presence of ATP, uvsX bind with
oligonucleotides cooperatively, upon ATP hydrolysis, the nucleoprotein
disassembles and uvsX is displaced by gp32, but uvsY
can assist uvsX rebind with oligonucleotides. The stable
nucleoprotein search on the double-stranded DNA and promote strand exchange
at homologous sites with the displaced strand that will be stabilized by
gp32. Then the oligonucleotides are extended by DNA polymerase
with strand displacement activity and a single-stranded DNA was
released.
Results
Stoichiometry of binding oligonucleotides by RecA
It was reported that RecA and ssDNA could form a compressed nucleoprotein
complex in the absence of ATP. The complex is inactive for strand exchange,
while in the presence of ATP the nucleoprotein will extend to functional
structure to perform strand exchange30. In addition, there was a
constant stoichiometry ratio between RecA and nucleotides for forming
nucleoprotein. To begin with, we demonstrated the ssDNA binding activity and the
stoichiometry of RecA either purchased or expressed by ourselves
(Protocol S1) using gel mobility shift assay31. As we
can see, RecA and ssDNA (54 nt) indeed formed nucleoprotein
and generated a low mobility band in the native agarose gel in the absence of
ATP (lane 1, Fig. 2A). However, RecA disassemble
from ssDNA when ATP was added (lane 2, Fig. 2A), which
could be caused by ADP produced from hydrolysis of ATP as RecA/ssDNA has
the strong ATPase activity. This assumption was verified by adding ADP into the
reaction, where we found that RecA disassemble from ssDNA when ADP was
added (lane 3, Fig. 2A). To prevent disassemble of the
nucleoprotein we introduced a modified nucleotide
adenosine-5′-o-(3-thio-triphosphate) (ATPγS) which could
not be hydrolyzed by RecA. By incubating various concentration of
RecA with ssDNA (12 pmol) and then analyzed on native
agarose gel, the corresponding binding ratio of ssDNA by RecA was
obtained. Through calculation, we obtained the average stoichiometry of about 3
nucleotides per RecA in the presence of ATPγS (Fig. 2B). In the same way, the stoichiometry of about 5 nucleotides
per RecA was obtained in the absence of ATP (Figure S1B), consistent with previous
research32333435. Therefore, in the following
experiment RecA was used to completely cover ssDNA based on the
3 nt/RecA in the presence of ATP and
5 nt/RecA in the absence of ATP.
Figure 2
(A) 160 pmol RecA was incubated with
12 pmol 54 nt oligonucleotides in the presence of
different nucleotide cofactor. Lane 1, no nucleotide. Lane 2, ATP. Lane 3,
ADP. Lane 4, ATPγS. Lane 5, no RecA was added. (B)
Incremental concentration of RecA was incubated with
12 pmol 54 nt oligonucleotides in the presence of
ATPγS. Lane 1–6 correspond 20, 40, 80, 120, 160,
0 pmol RecA was added respectively. (C) Schematic
of the process of strand exchange promoted by RecA. RecA and
isotope-labeled ssDNA (ss) can form a nucleoprotein complex, then
this complex will recognize its homologous double-stranded DNA (ds)
and displace the identical strand to form a new isotope-labeled
heteroduplex. RecA will disassemble from the product upon ATP
hydrolysis and recycle. (D) Result of RecA promoted strand
exchange between ssDNA oligonucleotides and homologous double-stranded DNA,
reaction details could be found in Materials and Methods except the
nucleotides cofactor variation: Lane 1, no nucleotides; Lane 2,
1 mM ATP; Lane 3, 1 mM ATP with 10 mM
phosphocreatine and 1 U creatine kinase; Lane 4,
5 mM ATP; Lane 5, 5 mM dATP; Lane 6,
5 mM ATPγS; Lane 7, no RecA; Lane 8 and 9 are
isotope-labeled ds and ss as markers.
RecA promote exchange between oligonucleotides with homologous
double-stranded DNA
As nearly all the nucleic acid detection methods depend on hybridization of
primer or probe with template, we then check the capability of nucleoprotein
complex formed by RecA and ssDNA to substitute the identical strand of
the homologous double stranded DNA. Here we designed an experiment to
demonstrate the strand exchange activity of RecA, as shown in Fig. 2C: The single stranded DNA (ss) was
isotope-labeled, which could form nucleoprotein with RecA. If the complex
(RecA/ss) could invade into homologous double stranded DNA
(ds), the isotope-labeled ds should be detected based on the
native PAGE analysis. So strand exchange of ssDNA oligonucleotides and their
homologous double stranded DNA was tested in our experiment. As illustrated in
Figure S2C, no isotope-labeled
dsDNA products was detected in the absence of ATP (lane 3, Figure S2C), while the exchanged dsDNA
containing isotope-labeled ss was observed on the native PAGE in the
presence of ATP and the exchange efficiency increased as the ATP concentration
increased (lane 4–9, Figure
S2C), which verified the DNA strand-substitution catalyzed by
RecA requires ATP as cofactor. However, the efficiency of strand
exchange was very low in the presence of 1 mM ATP, which could be
caused by the hydrolysis of ATP by RecA in the presence of ssDNA. As
RecA can form stable nucleoprotein with ssDNA in the presence of
ATPγS as shown in the experiment above, we wonder if
ATPγS can replace ATP to increase the efficiency. However, when
ATPγS was employed, no exchange products were obtained (lane 6,
Fig. 2D). Those results implied that ATP hydrolysis
was indispensable in the process of strand exchange promoted by RecA.
Therefore, It was supposed that the low efficiency of strand exchange was caused
by hydrolysis of ATP by RecA. It is well known that, RecA
hydrolyze ATP into ADP continuously when it bind with ssDNA, so in all the
strand-exchange reaction in vitro, an ATP regeneration system (composed
of phosphocreatine and creatine kinase) that convert ADP into ATP was included,
such as in RPA. When ATP regeneration system was introduced into the
reaction mixture with 1 mM ATP, the efficiency of strand exchange
between ssDNA oligonucleotides and homologous double-stranded DNA increased
dramatically (lane 3, Fig. 2D). However, the addition of
ATP regeneration system made the reaction more complex and costly. We are very
glad to found that this problem could be solved through increasing the
concentration of ATP. In the presence of 5 mM ATP, the exchanging
efficiency reach to the same level with the reaction containing ATP regeneration
system (lane 4 vs. lane 3 in Fig. 2D). It has been
reported that dATP is a better cofactor for RecA36.
Therefore, we investigate the feasibility to exchange the ATP in our system with
dATP. As illustrated in Fig. 2D, the efficiency of strand
exchange catalyzed by RecA in the presence of dATP (lane 5) was as same
as that in the presence of ATP (lane 4). Besides, the capacity to perform strand
exchange of ssDNA of varying length based on this system was investigated,
revealing that ssDNA as short as 24 nt was enough for RecA
promoted strand exchange (Figure
S2B). In short, we realized the opening of dsDNA and substitution with a
ssDNA by using RecA of E. coli. And we found that ATP hydrolysis
was essential for the whole process of strand exchange. The ATP regeneration
system could be eliminated by using high concentration of ATP. Moreover, dATP
could be applied as cofactor for RecA to perform strand exchange between
short ssDNA and homologous double stranded DNA with same efficiency.
Ligation of two oligonucleotides after strand exchange
As research showed that RecA remain associated with the heteroduplex after
strand exchange37, so after strand exchange, what we care about
is whether 3′-OH terminal of the invasion strand can be manipulated
by DNA modifying enzyme like DNA ligase. Some isothermal detection methods like
RCA adopt the strategy of ligation to initiate the nucleic acid
detection. Therefore, we designed the experiment to verify the feasibility of
ligation reaction of two ssDNA in the presence of duplex template with the aid
of RecA-based dsDNA opening system. As shown in Fig.
3A, we designed two ssDNA oligonucleotides that were complementary to
one strand of the duplex template in juxtaposition. The first one was labeled
with isotope and the second one with 5′-phosphate group that is
necessary for ligation reaction catalyzed by T4 DNA ligase. Then the
nucleoprotein complexes formed by two oligonucleotides with RecA could
scan double stranded template and invade at the homologous sites to form
hetroduplex with a nick in the middle, which would be recognized and ligated by
T4 DNA ligase to yield an isotope-labeled product with expected length. However,
the ligation efficiency was very low in the presence of high concentration of
ATP (lane 1, Figure S4B). We
speculated that after nucleoprotein complex invaded into duplex template to form
D-loop the displaced strand was likely to re-anneal with the complementary
strand and exclude the invasion ssDNA oligonucleotides before they were ligated
by T4 DNA ligase. Previous studies reported that single-stranded DNA binding
protein (SSB) can aid in the formation of nucleoprotein complexes and
stimulate DNA strand exchange by binding to the displaced single-stranded
DNA383940. Single-strand DNA-binding protein (SSB)
is a 178-amino-acid-long protein found in E. coli that binds to
single-stranded regions of DNA. It has important function during all aspects of
DNA metabolism: replication, recombination, and repair. As well as stabilizing
the single-stranded DNA, SSB proteins bind to and modulate the function
of numerous proteins involved in all of these processes. Moreover SSB
protein is easily obtained from commercial sources or direct expression from
E. coli (Protocol S1 and Figure
S3). When SSB was introduced into the reaction, the efficiency
of ligation increased greatly (lane 2, Figure S4B). Out of expectation, when dATP was employed into the same
reaction, the ligation efficiency was further improved (Fig.
3B). As it is well known that ATP is a cofactor of T4 DNA ligase and
studies showed that although adenylation enzyme could form in the presence of
dATP, it is inactive in the ligation reaction41. However, it is
surprising to find that dATP could also serve as a cofactor for T4 DNA ligase to
work in the condition employed in our experiment (Figure S5). Eventually, we had performed
ligation of two oligonucleotides using double-stranded DNA as template at a
constant temperature. This would be a great help for the isothermal detection
methods which rely on ligation reaction such as rolling circle amplification
(RCA) to realize the direct detection of double-stranded DNA
isothermally.
Figure 3
(A) Schematic of the process of RecA mediated ligation of two
ssDNA oligonucleotides using double-stranded DNA as template. Firstly,
RecA bind with two ssDNA oligonucleotides to form nucleoprotein
complex respectively to recognize and unwound double-strand template
homologously. Then, the two oligonucleotides annealed with complementary
strand in juxtaposition and are ligated by T4 DNA ligase. (B) PAGE
analysis of RecA mediated ligation reaction: Lane 1, the reaction was
conducted in presence of dATP. Lane 2, RecA was not included. Lane 3,
RecA was included while the double-stranded DNA template was removed. Lane 4
and 5, 32P-labeled 108 nt and 54 nt
oligonucleotide as markers.
Primer extension after strand exchange
Besides ligation, most of the isothermal detection methods, such as SDA
and LAMP and so on, rely on generation of single stranded DNA as target,
which could be served as template of the primers for DNA polymerase to start the
isothermal amplification. So we wonder if the 3′-OH terminal of the
invasion strand can be recognized by the DNA polymerase with strand displacement
activity, like Bst and Bsm DNA polymerase, to displace one strand of the duplex
template after extension. In order to figure out the accessibility of the
3′-OH terminal of the invasion strand by the DNA polymerase, we
designed a 5′-ssDNA tailed duplex DNA to serve as template (left,
Fig. 4A). In the presence of RecA and ATP,
almost all the labeled primers were extended to corresponding length (lane 3,
Fig. 4B). However, in the absence of RecA, only
a little background products were observed (lane 4, Fig.
4B). Therefore, it can be concluded that the 3′-OH
terminal of the primer was accessible for DNA polymerase to elongate after
strand exchange. However, the natural DNAs are always intact duplex, unlike the
case of 5′-ssDNA tailed duplex DNA where the displaced strand was
completely stripped off the heteroduplex. As shown in Fig.
4A (right), after RecA assisted the ssDNA oligonucleotide to
invade into intact duplex to form D-loop, the displaced strand was not
completely dissociated and the downstream still paired42434445. This structure was not stable because the primer
may be excluded through re-annealing of the displaced strand as referred above.
So we designed an blunt-ended duplex as a target to explore if the polymerase
could recognize at the 3′-OH terminal and overcome the barrier of
downstream base-pair through displacing it (right, Fig.
4A). In the presence of RecA, almost half of the labeled primers
were extended to corresponding length (lane 1, Fig. 4B),
while in the absence of RecA only a little products were obtained as
background (lane 2, Fig. 4B). The results revealed that
isotope-labeled primer have invaded into double-stranded template, and it could
be extended by the DNA polymerase with strand displacement activity to release a
ssDNA. Although the efficiency of extension using blunt-ended duplex as template
was lower than that of 5′-ssDNA tailed duplex DNA, it can be
concluded that strand exchange promoted by RecA is compatible to DNA
polymerase with strand displacement activity and ssDNA will be released in the
process of DNA replication.
Figure 4
(A) Schematic of the process of primer extension after strand exchange
on 5′-ssDNA tailed duplex and intact blunt-ended duplex
template. Left, after complete strand substitution of the isotope-labeled
primer with one strand of the 5′-ssDNA tailed duplex, the
isotope-labeled primer was elongated by DNA polymerase. Right, after strand
exchange of isotope-labeled primer with one strand of blunt-ended duplex,
D-loop formed. Then the isotope-labeled primer was extended by DNA
polymerase with strand displacement activity and a single-stranded DNA was
released (B) Results of primer extension after strand exchange. Lane
1, intact blunt-ended duplex served as template in the presence of
RecA. Lane 2, intact blunt-ended duplex served as template in the
absence of RecA. Lane 3, 5′-ssDNA tailed duplex served as
template in the presence of RecA. Lane 4, 5′-ssDNA tailed
duplex served as template in the absence of RecA. Lane 5,
isotope-labeled primer was extended on the complementary 78 nt
single-stranded template to serve as a positive control. Lane 6,
32P-labeled 78 nt oligonucleotide. Lane 7,
32P-labeled 54 nt oligonucleotide as marker
respectively. (C) Schematic of RecA based DNA amplification.
First, single-stranded primers bind with RecA to form nucleoprotein
complex, which could scan the double-stranded template until the homologous
sites are located. Then, following strand exchange, the displaced strand is
stabilized by SSB and primers are extended by Bsm DNA
polymerase. After extension, two ssDNA are generated. (D) Results of
RecA-based DNA amplification using blunt-ended duplex as
template. Lane 1, in the presence of 5 mM ATP. Lane 2, in the
presence of 5 mM dATP. Lane 3 and 4 are 54 nt and
118 nt 32P-labeled oligonucleotides as marker
respectively.
The RecA based DNA amplification
We have obtained ssDNA through RecA promoted strand exchange followed by
extension of the invading strand with DNA polymerase. However, the yield was not
very high (lane 1, Fig. 4B). So we wonder if the displaced
ssDNA can serve as template for another ssDNA primer, the amplification of
templates should carry on (Fig. 4C). As a result, more
ssDNA for isothermal amplification template could be produced in the process of
amplification, which would be a great advantage for isothermal detection
methods. However, no amplification products were obtained in the presence of ATP
(lane 2, Figure S6B). We deduced
that when two primers were used, a lot of ssDNA that were complementary to each
other were generated. As mentioned before, SSB can be used to bind with
these ssDNA which could serve as template for the primers before they annealed
to each other. Consistent with our expectations, amplification products were
obtained when SSB was employed (lane 1, Figure S6B). However, the efficiency of
amplification was still not very high, we speculated that RecA remain
associated with the heteroduplex after strand exchange37 and the
homologous sites could be open by nucleoprotein complex only when RecA
dissociated from the heteroduplex by hydrolysis of ATP. This may be improved by
adding dATP, which was hydrolyzed faster than ATP36. It was very
glad to find that in the presence of dATP the amplification efficiency greatly
increased (lane 2, Figure 4D). Besides, we demonstrated oligonucleotides with
54 nt or 35 nt in length could all be used as primers
for amplification of blunt-ended duplex(Figure S6C). In addition to blunt-ended duplex, plasmid DNA could
also serve as template for RecA based DNA amplification, and the
amplification products were also visible on stained native agarose gel (Figure S7). Through analysis on
multifunctional laser scanning imaging system, we calculated that the templates
were amplified 240 times, which implies that more than 240 fold ssDNA were
produced in the process of amplification. Although previous research have
established an amplification method which can target double-stranded DNA
isothermally by introducing recombinase from T4 phage20. However,
as mentioned before, the proteins they used were all from T4 phage and
unavailable commercially. Besides, recombinase would continuously hydrolyze ATP,
so an ATP regeneration system should be included. Here, by using commercially
available recombinase of E. coli (RecA), we realized the multiplex
ssDNA templates could be produced and have eliminated the need for ATP
regeneration system by introducing dATP.
Discussion
In summary, we have put forward a simple solution for opening double-stranded DNA for
isothermal detection methods through invasion of ssDNA into double-stranded DNA in
assist of RecA protein of E. coli. After the ssDNA annealed with
complementary strand of the double-stranded template, it can be manipulated by other
DNA modified enzyme like DNA ligase and DNA polymerase. The RecA-based dsDNA
opening system described here appears to have several promising features for
research and diagnostic applications as follows: All proteins (RecA and
SSB) used in our method are commercially available, and they can be
expressed easily in ordinary laboratory for large-scale preparation; RecA has
been reported to promote strand exchange reaction with a high sequence
specificity46, so once combined with other isothermal
amplification strategies it could improve the specificity of whole method; The ATP
regeneration system is eliminated in our system, which make this method simple and
cost-efficient. Moreover, dATP could serve as the cofactor of RecA to perform
strand exchange in place of ATP, offering more flexibility to our system; After the
strand exchange, the 3′-OH terminal of the invasion strand was proved to
be accessible to other DNA modifying enzymes like DNA ligase or polymerase, which is
compatible with almost all reported isothermal detection methods. By designing a
padlock probe with two binding arms complementary to one strand of double stranded
template in juxtaposition, rolling circle amplification (RCA) can detect
dsDNA18. Based on our solution, starting structure of
loop-mediated isothermal amplification (LAMP) can produce at a constant
temperature21 and the double-stranded DNA with Nickase site at
both ends are obtained using only one pair of primers at a constant temperature16. By introducing T7 promoter sequence on the 5′ terminal
of primers, Nucleic Acid Sequence Based Amplification (NASBA) can conduct
using dsDNA as substrate15. Therefore, The RecA-based dsDNA
opening system described here is a general solution to open dsDNA, serving as a
platform to develop more isothermal nucleic acids detection methods for real DNA
samples.
Materials and Methods
Oligonucleotides, enzymes, and other reagents
All oligonucleotides were purchased from Sangon Biotech (Shanghai, China) and are
shown in Table S1. Bsm DNA Polymerase (Large Fragment), T4 polynucleotide kinase
were purchased from Thermo Scientific. Plasmid pET-28(a) was purchased from
Novagen, now part of Merck Biosciences. Trans5α Chemically Competent
Cell, BL21(DE3) Chemically Competent Cell, FastPfu DNA Polymerase and dNTP were
purchased from TransGen Biotech (Beijing, China). Ni–agarose His tag
protein purification kit was bought from Beijing CoWin Biotech.
[γ-32P]ATP was purchased from Furui Biological
Engineering (Beijing, China).
Labelling Reaction
A reaction mixture containing oligonucleotides X1 and X1-35 with
50 mM Tris-HCl (pH 7.8), 40 mM NaCl, 10 mM
MgCl2, 1 mg/mL BSA, 10 μCi
[γ-32P]ATP and 10 units of Polynucleotide kinase
(PNK) was incubated for 1 h at 37 °C for DNA
phosphorylation. The labelled product was purified by 10% denaturing
polyacrylamide gel.
DNA binding assays
Reactions were performed by incubating indicated concentration of purified
proteins with 12 pmol X1 (Table S1) at 37 °C
for 10 min. Standard conditions were 25 mM Tris (pH
7.6), 1 mM Magnesium chloride and 1 mM DTT. The reaction
volume of all binding assays was 10 μl. After the
reaction, 2.5 ul 6* loading buffer (0.25% bromophenol blue, 36%
sucrose and 30 mM EDTA) was added into each tube. Subsequently, all
the samples were loaded on 2% native agarose gel. The results were analyzed by
Typhoon FLA 7000 IP and the stoichiometry of RecA to oligonucleotides was
determined through calculation (GE Healthcare).
DNA exchange assays
Incubate 0.05 μM 32P-labelled
oligonucleotides X1 with 18 pmol RecA that completely cover
the ssDNA oligonucleotides based on the stoichiometry in the standard condition
as follows: 25 mM Tris (pH 7.6), 10 mM Magnesium
chloride, 1 mM DTT, nucleotide cofactors used were as shown in the
Figure. Then 0.05 μM homologous double-stranded DNA
formed by annealing of the same unlabeled oligonucleotides X1 with their
complementary strand X1C (Table S1) was added. When ATP regeneration system was
included, phosphocreatine was 15 mM, creatine kinase was
1 U. The reaction volume was 10 μl. The
incubation last for 10 min at 37 °C. After
the reaction, the mixture was extracted by phenol-chloroform and precipitated
with ethanol. The sediment was dried by Vacuum Drier and loaded on 12% native
polyacrylamide gel. The results were analyzed by Typhoon FLA 7000 IP (GE
Healthcare).Incubate 0.05 μM 32P-labelled X1 and
0.05 μM 5′-phosphorylated X1f with
18 pmol RecA in condition as follows: 25 mM Tris
(pH 7.6), 10 mM Magnesium chloride, 1 mM DTT, nucleotide
cofactors used were as shown in the Figure. Then 0.05 μM
double-stranded DNA(formed by annealing of T1 and T2), 15 pmol
SSB, 5 U T4 DNA ligase was added followed by incubating
for 1 h. After that, 1% SDS and 1 U proteinase K were
added and incubated for another 15 min. Afterwards, the reactions
were extracted by phenol-chloroform and precipitated with ethanol. The sediment
was dried by Vacuum Drier and loaded on 10% denaturing polyacrylamide gel. The
results were analyzed by Typhoon FLA 7000 IP(GE Healthcare).
Extension after DNA exchange
We designed a 5′-ssDNA tailed duplex DNA which was formed by
unlabeled X1 annealed with X3 and a blunt-ended duplex DNA annealed with X3 and
X4 (Table S1). First, we demonstrated 32P-labelled X1 can
substitute the unlabeled X1 in the 5′-ssDNA tailed duplex DNA and
extended by DNA polymerase. The reaction condition were as follows:
25 mM Tris(PH 7.6), 10 mM Magnesium chloride,
5 mM ATP, 0.25 mM dNTP, 210 pmol
RecA, 4 U Bsm, 1 mM DTT. Primer and template used
in this reaction were 32P-labelled X1
0.05 μM, 5′-ssDNA tailed duplex DNA
0.05 μM. Then, we demonstrated
32P-labelled X1 can exchange with the blunt-ended duplex and
extended by DNA polymerase with strand displacement activity. The reaction
condition were as follows: 25 mM Tris(PH 7.6), 10 mM
Magnesium chloride, 5 mM ATP, 0.25 mM dNTP,
210 pmol RecA, 4 U Bsm, 1 mM DTT.
Primer and template used in this reaction was 32P-labelled X1
0.05 μM, blunt-ended duplex
0.05 μM. After incubation at
37 °C for 1 h, the reactions were extracted
by phenol-chloroform and precipitated with ethanol. The sediment was dried by
Vacuum Drier and loaded on 10% denaturing polyacrylamide gel. The results were
analyzed by Typhoon FLA 7000 IP(GE Healthcare).
Amplification using two primers
Pre-incubation of the mixture of 25 mM Tris(pH 7.6), 8%
(m/v)PVP(Polyvinyl pyrrolidone), 6 mM Magnesium chloride,
1 mM DTT, 420 pmol RecA,
0.3 μM forward primer X1, 0.3 μM
reverse primer X1-re and 5 mM nucleotide cofactors shown in the
Figure for 5 min at 37 °C. Subsequently the
mixture of double-stranded template formed by annealing of T1 and T2
(blunt-ended duplex), 250 μM dNTP, 360 pmol
SSB and 4 U Bsm was added, the final concentration of
template was 625 pM. The incubation continued at 37 °C
for 1 h and the reaction was extracted by phenol-chloroform and
precipitated with ethanol. The sediment was dried by Vacuum Drier and loaded on
10% denaturing polyacrylamide gel or 4% agarose gel. The results were analyzed
by Typhoon FLA 7000 IP(GE Healthcare).
Additional Information
How to cite this article: Chen, G. et al. A general solution for
opening double-stranded DNA for isothermal amplification. Sci. Rep.
6, 34582; doi: 10.1038/srep34582 (2016).
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