Intrinsic bent DNA sites in the chromosomal replication origin of Xylella fastidiosa 9 a 5 c

The features of the nucleotide sequences in both replication and promoter regions have been investigated in many organisms. Intrinsically bent DNA sites associated with transcription have been described in several prokaryotic organisms. The aim of the present study was to investigate intrinsic bent DNA sites in the segment that holds the chromosomal replication origin, oriC, of Xylella fastidiosa 9a5c. Electrophoretic behavior analyses, as well as in silico analyses of both the 2-D projection and helical parameters, were performed. The chromosomal segment analyzed contains the initial sequence of the rpmH gene, an intergenic region, the dnaA gene, the oriC sequence, and the 5' partial sequence of the dnaN gene. The analysis revealed fragments with reduced electrophoretic mobility, which indicates the presence of curved DNA segments. The analysis of the helical parameter ENDS ratio revealed three bent DNA sites (b1, b2, and b3 ) located in the rpmH-dnaA intergenic region, the dnaA gene, and the oriC 5' end, respectively. The chromosomal segment of X. fastidiosa analyzed here is rich in phased AT tracts and in CAnT motifs. The 2-D projection indicated a segment whose structure was determined by the cumulative effect of all bent DNA sites. Further, the in silico analysis of the three different bacterial oriC sequences indicated similar negative roll and twist >34.00° values. The DnaA box sequences, and other motifs in them, may be associated with the intrinsic DNA curvature.


Introduction
After the structure of DNA was solved (1), it was proposed that DNA molecules could exist in several structural conformations (2).The discovery of alternative structures, such as curvature in the promoter and replication origins that were either induced by the intrinsic DNA sequence or produced by DNA flexibility, permitted the establishment of a relationship between structure and function (3).
Intrinsic bent DNA sites are usually caused by adenine/ thymine-rich tracts that are in phase with helical repeat ~10. 5 base pairs (bp) (4).Alternatively, flanking sequences can have a significant influence on DNA conformation; some curvatures have been described in the absence of A/ T (5).
Investigation of the nucleotide sequences of Archaebacteria has revealed that genomic DNA sequences of replication initiation contain similarities, as described for eukaryotes (16).The replication origins of prokaryotes and lower eukaryotes are located in specific DNA sequences that are always found at the same site of the chromosome.These sequences are by definition segments of DNA necessary and sufficient for molecular replication (17).Specific protein-binding sequences in prokaryotic replication sites can present conserved structural domains such as curved DNA, which plays an important role in DNA replication (18).
Xylella fastidiosa 9a5c is a Gram-negative microorganism that causes citrus variegated chlorosis disease in citrus trees (19).The complete genome sequence of strain 9a5c has been reported (20).The replication origin, which controls the duplication of the single chromosome of X. fastidiosa, contains AT-rich segments, five putative DnaA box sequences (R1-R5), and a box of 24 nucleotides with eight ACC repetitions (21).The box of 24 nucleotides replaces the traditional box of 13 nucleotides reported for the Escherichia coli chromosome (22).These regions are important for both protein-binding and the opening of DNA in the bacterial replication process.A report, which states that the genetic transformation of X. fastidiosa 9a5c is possible only with plasmids building from the chromosomal X. fastidiosa replication origin (21), suggests that this oriC has an essential feature that other oriC lack.Thus, the evidence implies that this chromosomal origin is essential for the X. fastidiosa transformation system and is structurally different from the E. coli origin consensus.Thus, the aim of the present study was to map intrinsic bent DNA sites in the X. fastidiosa replication origin by electrophoretic behavior and by in silico analyses.In order to compare these results with other bacterial replication origins, we performed in silico analyses as 2-D projections and evaluated the roll and twist helical parameters in the oriC sequences of the X. fastidiosa strain Temecula1, Bacillus subtilis, and E. coli.

DNA fragments
The recombinant plasmids p16KdAori and p16Kori were kindly provided by Patrícia B. Monteiro (Fundação para a Defesa da Citricultura, Fundecitrus, Araraquara, SP, Brasil).These plasmids contain DNA fragments that include the replication chromosomal origin of X. fastidiosa (21).The clone p16KdAori was constructed in a pBluescript (pBS) plasmid, along with an insert of 4139 bp that contains the X. fastidiosa ribosomal operon promoter (rop), the gene for resistance to kanamycin (kan r ), and a fragment of 1892 bp.This fragment contains the initial sequence of the rpmH gene, a 141-bp intergenic region, the dnaA gene, the oriC region, and 24 initial nucleotides of the dnaN gene.The oriC fragment is restricted to the intergenic region dnaA-dnaN with 296 bp.The p16Kori clone contains the oriC within a 364-bp fragment.The recombinant plasmids p16KdAori and p16Kori were transformed in DH5α E. coli competent cells (23), and the plasmid DNA was purified by the CTAB method (24) and/or by alkaline lysis (23).After purification, the plasmids were cleaved with different restriction enzymes according to manufacturer instructions.

Electrophoretic analysis of fragments
The restriction subfragments were electrophoresed on 1% agarose gels (AGA) at room temperature and on 6% polyacrylamide (PA) gels at 4°C without ethidium bromide (EtBr).To confirm the presence of bent DNA, the samples were incubated overnight with 1 µg/mL EtBr and electrophoresed on previously run 6% PA gels with 1 µg/mL EtBr in the running buffer (PA + EtBr).EtBr acts locally between base pairs, abolishing the intrinsic DNA curvature and straightening the fragments (25).All gels were run in 1X TBE buffer (45 mM Tris-borate, 1 mM EDTA, pH 8.0), molecular weight marker 1-kb Ladder Invitrogen, stained after running with 0.1 µg/mL EtBr, and documented with a UVP BioImaging System, USA, under UV light.The gel concentration, running time, and running voltage were adjusted relative to the size of the fragments analyzed.The mobility pattern of each fragment was obtained by the calculation of the R-value (ratio of apparent/real fragment size observed in each gel system).R-values between 0.90 and 1.09 indicate no alterations in mobility, those higher than or equal to 1.10 indicate reduced mobility, and those lower than 0.90 indicate fast mobility (14,26).

In silico analysis of the curvature
In silico analysis of the DNA sequence curvature provided results that are compatible with electrophoretic data (18).In the present study, we used the dinucleotide wedge model of Bolshoy et al. (27) to predict the 3-D path of the 1892-bp DNA segment.The 2-D projection and structural parameters were calculated by Map15a and 3-D15m1 softwares (28), using the algorithm of Eckdahl and Anderson (18) and the helical parameters of Bolshoy et al. (27), as described by Pasero et al. (11) and Marilley and Pasero (29).Each plotted value takes into account the contribution of the surrounding nucleotides.Putative bent segments were identified using the ENDS ratio, which describes the ratio of the contour length of a fragment helical axis to the shortest distance between the fragment ends.The twist angle (horizontal rotation between 2 consecutive bp), variations of the roll angle (which estimates the rolling-open of the base pairs along their long axes) and ∆G values, which predict the stability of the DNA duplex, were calculated with the Map15a software.These calculations used a 120bp window width and a 10-bp step for the 1892-bp segment, as well as a 30-bp window width and a 10-bp step for Intrinsic bent DNA in X. fastidiosa oriC www.bjournal.com.br the oriC segments from X. fastidiosa 9a5c (NC_002488), X. fastidiosa strain Temecula1 (NC_004556), Bacillus subtilis (NC_000964), and E. coli (AC_000091).
By convention, if base pairs open toward the minorgroove side, the roll angle is positive.Conversely, negative roll angles that cause a narrow minor groove suggest a bent region (30).The 3-D15m1 software was used to obtain both the 2-D projection of the 3-D fragment trajectory and the ∆G values.

Electrophoretic mobility
Restriction fragments of the p16KdAori and p16Kori clones were analyzed by electrophoresis on AGA gels, PA gels, and PA + EtBr gels.On PA gels, the migration of DNA fragments was dependent on both size and structure.
Fragments containing bent DNA segments migrated through the mesh of this gel with lower or higher apparent molecular sizes than expected from the fragment length.In contrast, the migration of fragments through AGA gels, which form an irregular mesh, is dependent only on their size.The PA gels confirm the presence of bent DNA sites in fragments.EtBr on these gels intercalates between the DNA base pairs and the fragments, abolishing DNA curvature, and thus the fragments have a regular mobility in this gel.In the p16KdAori clone, the restriction enzymes EcoRI, BamHI and XbaI did not cut the rop promoter sequence or the kan r gene, keeping the remaining insert linked to the pBS plasmid (Figure 1, black arrow on gels).Double digestion with the BamHI + XbaI produced two subfragments: one 997-bp fragment containing the initial sequence of the rpmH gene, the 141-bp intergenic region, and part of the dnaA gene, and a second 895-bp fragment that contains Figure 1.Analysis of the electrophoretic mobility of the oriC chromosomal segment from Xylella fastidiosa 9a5c.The restriction map of the p16KdAori (7100 bp) clone is at the top.The numbers above each fragment are the R-values.White vertical and horizontal arrows indicate fragments with reduced mobility, with R-values ≥1.10; black horizontal arrows represent a fragment that contains the ribosomal operon promoter (rop) and the gene for resistance to kanamycin (kan r ), which remain linked to the plasmid pBluescript (pBS) in this restriction enzyme cleavage.M = molecular weight marker 1-kb Ladder; AGA = 1.0%agarose gel; PA and PA + EtBr = 6% polyacrylamide gels without and with ethidium bromide, respectively.The white rectangle on the PA gel corresponds to the 997-and 895-bp fragments which run together, because the 895-bp fragment has a reduced electrophoretic migration (Rvalue 1.10).Lane 1, BamHI (B) + XbaI (X); lane 2, EcoRI (E) + BamHI (B) restriction sites.The 364-bp fragment (Figure 2, lane 1, white arrow), which contains the X. fastidiosa oriC replication origin, presented reduced electrophoretic mobility (R-value 1.12).

Bent structure
The sequence of the 1892-bp fragment was analyzed with the Map15a software for helical curvature parameters, and with the 3-D15m1 software for 2-D projection.The helical parameters of ENDS ratio, ∆G value, roll angle, and twist angle confirmed the presence of the bent DNA sites at the 160-(b1), 860-(b2) and 1570-bp (b3) positions (Figure 3).The highest ENDS ratio value, 1.19, was observed for the b1 bent DNA site within the 290-bp fragment (BamHI/EcoRI).This site is located in the intergenic region between the rpmH and dnaA genes, a region with a negative roll angle (-0.15) and a twist angle greater than 34.00°( 34.08°).The DNA bent site b2 was located at the end of the 621-bp fragment.This site showed the smallest ENDS ratio value 1.13, a twist angle of 34.11°, and a higher negative roll angle of -0.34.The X. fastidiosa oriC replication site presented the bent DNA site b3, with an ENDS ratio value of 1.16, a roll angle of -0.77 (the most negative the 3' end of the dnaA gene, the oriC origin, and the initial sequence of the dnaN gene (Figure 1, lane 1).On PA gels, these two fragments migrate with the same mobility (Figure 1, lane 1, rectangle) because the 895-bp fragment has a reduced migration (R-value 1.10, lane 1, white arrow).This same clone was cleaved with the enzymes EcoRI/ BamHI (Figure 1, lane 2), and the 621-bp EcoRI subfragment presented normal migration on PA gels (R-value 0.90).The 290-and the 981-bp fragments had a significant reduction of mobility on PA gels (Figure 1, lane 2, white arrows), with R-values of 1.19 and 1.12, respectively.
The 981-bp fragment (Figure 1, lane 2), which is 86-bp longer than the 895-bp fragment (Figure 1, lane 1), did not show a total return to its real molecular weight on the PA + EtBr gel.This effect may be due to transitory formation of the alternative cruciform structures on the left side of this segment.Structures other than bent DNA are not affected by EtBr, which can explain the electrophoretic behavior observed for the 981-bp fragment on the PA + EtBr gel.
The p16Kori clone was cleaved with the restriction enzymes SmaI + BamHI (Figure 2, lane 1).The 1300-and 803-bp fragments contain the rop promoter and kan r gene.
Intrinsic bent DNA in X. fastidiosa oriC www.bjournal.com.brsupercoiling value), and a twist angle greater than 34.00°( 34.07°).The lowest ∆G value was observed for the bent DNA site b3.
Negative roll angles, that cause a narrow minor groove, suggest a bent region that, associated with a twist parameter of >34.00°, indicates curved negative supercoiling DNA.This structure has been reported to have high affinity for proteins such as DnaA (31).These parameters suggest that the bent DNA site b3 is actively involved in oriC activity.
The 2-D projection of the 1892-bp fragment was obtained using the 3-D15m1 software (Figure 4), which allows the visualization of the global structure of the fragment produced by the cumulative effect of the bent sites b1, b2, and b3.We observed low ∆G values (227, 219 and 207, respectively), which arise from the AT-rich tracts (Figure 4, black rings).Five putative DnaA boxes (R1-R5) and the eight ACC repetition box with 24 nucleotides previously reported (21) are located in this region.The rotation of the fragment sequence by 30° and 60° confirms that the bent sites are important for the maintenance of the shape of these fragments and should be essential for the maintenance of the function of these regions.

Nucleotide sequence analysis
Intrinsic bent DNA sites occur in regions containing tracts of adenine/thymine phased with the DNA helix turn ( ~10.5 bp).The CAnT motif is located either in the center or near the curvature and seems to be responsible for high bent peak formation (7).For the analysis of the nucleotide sequences in the bent DNA sites described in the present study, we confirmed the DNA helix turn phasing of two or more adenine/thymine tracts, which were located around the sites, and the presence of the CAnT motifs.Figure 5 shows the three bent DNA sites, b1, b2, and b3, in which the curvature peak is represented by a square.The b1 site, located in the intergenic region between the rpmH and dnaA genes, is flanked by CAnT motifs (double underlined).The b2 site, located inside the dnaA gene, is formed by phased AT tracts (underlined) and by an upstream CAnT motif (double underlined).The b3 site, located at the 5' end of the oriC, is also formed by A and/or T phased tracts (underlined).The GATC motif (Figure 5, bold and italic) was observed to be distributed in the sequence analyzed.
A detailed analysis of the oriC replication origin in X. fastidiosa shows the previously described AT-rich tracts with 16 nucleotides (bold), five DnaA boxes (R1-R5), and 24 nucleotides of the ACC repetition box (bold and underlined).In the present study, we identified a motif containing four tracts of six nucleotides called ATP-dependent DnaA box (Figure 5, wavy lines) (32).

oriC DNA curvature
In order to confirm the structural aspects of oriC among related prokaryotes, 2-D modeling of the 3-D DNA path, the ENDS ratio, and the roll and twist helical parameters were obtained for the nucleotide sequence of the replication origins from X. fastidiosa 9a5c, X. fastidiosa Temecula1, B. subtilis, and E. coli (33).We used the Map15a software to assess helical curvature parameters and the 3-D15m1           For each origin, we identified the positions of the most prominent curvature peaks with circles in the 2-D projection.The X. fastidiosa 9a5c origin sequence shows two main peaks in the ENDS ratio: 1.06, located before the first DnaA box at the 36-bp position, and 1.07, located between the first and second DnaA boxes at the 117-bp position (Figure 6A).The observed ENDS ratios for the X. fastidiosa Temecula1 origin were: 1.06, located before the first DnaA box at the 36-bp position, and 1.07 located within the second DnaA box at the 117-bp position (Figure 6B).For B. subtilis, we identified two prominent ENDS ratio peaks located at positions 90 and 147 bp.These two peaks show the same ENDS ratio value of 1.04, with the first located Figure 6. Figure 6. Figure 6. Figure 6. Figure 6.In silico analysis of the bacterial oriC.The nucleotide sequences from Xylella fastidiosa 9a5c (A), X. fastidiosa Temecula1 (B), Bacillus subtilis (C), and Escherichia coli (D) are described in DoriC, a database of the oriC region in bacterial genomes (33).The 3-D15m1 software was used for 2-D projection, and the helical curvature parameters (ENDS ratio, twist angle, and roll angle) were calculated using the Map15a software with a 60-bp window width and a 10-bp step.The ENDS ratio positions are indicated by a circle in the 2-D projection.
between the second and third DnaA boxes and the second located after the third DnaA box (Figure 6C).The E. coli origin (Figure 6D) shows three prominent ENDS ratio peaks with 1.03 values, as well as two others with a value of 1.02.The first, at the 90-bp position, is located between the second and third DnaA boxes.The other four peaks (at the 183-, 234-, 270-, and 315-bp positions) are located after the third DnaA box.
The replication origins of these four organisms were analyzed by the roll and twist helical parameter values (Figure 6A-D).There is a predominance of negative roll angle, in addition to twist values above 34.00°, at the same position as the ENDS ratio peaks described for all oriC analyzed.

Discussion
Electrophoretic and in silico analysis revealed that the 1892-bp fragment analyzed in the present study, which contains the chromosomal replication origin (oriC ) of X. fastidiosa, showed intrinsic bent DNA sites.The R-values (1.19, 1.12, and 1.10) are in accordance with all described bent DNA sites, which are greater than or equal to 1.10 (34).The electrophoretic behavior of these fragments is consistent with the 3-D modeling, which shows the presence of sequence-directed curvature.
In silico analysis of this fragment showed at least three bent sites at the 160-(b1 ), 860-(b2 ), and 1570-bp (b3 ) positions, all with ENDS ratio values higher than 1.11.The b1 site is located in the promoter region of the dnaA and rpmH genes, and can play a role in the transcription of these genes.The b2 site is located inside the dnaA gene.There is no explication for this location, since bent DNA sites have only been described in promoters, intronic regions, and replication origins (14).The b3 site is located in the replication origin of X. fastidiosa and may be involved in the replication process of this bacterium's chromosomal DNA.Regarding the bent DNA site b3, its relationship with the dnaN gene promoter is difficult to establish because it is located -293 bp from the starting point of this gene.It has been reported that a bent DNA site upstream of the prokaryotic promoter is always located at -50 to -200 bp (30).
ENDS ratio values of 1.15 or higher were defined as indicative of bent DNA elements in the Bacillus thuringiensis chromosome, for which an average of eight ENDS ratio values yielding a mean greater than 1.2 for each 10-kb segment has been reported (35).However, ENDS ratio values lower than 1.10 were reported for the Xenopus laevis ribosomal intergenic sequence (36).On the basis of these results, it is clear that the ENDS ratio value contributes importantly to fragment curvature.Several peaks with lower ENDS ratios can determine a strongly curved segment.The length of the observed fragment and the calculation parameters, such as the window width and the interval steps, contribute to the establishment of the ENDS ratio value (30).
The helical parameters twist and roll angles were also evaluated for the replication origin of three additional bacterial oriC segments.We found negative roll angles ranging from -0.15 to -0.76 for this region, as well as twist angles ranging from 34.07° to 34.11°.These data show negative roll angles and twist angles above 34.00°, in agreement with curved regions with negative supercoiling, as described for regions with high affinity for the DnaA protein (31).According to Molina et al. (37), bending and supercoiling are requirements for the creation of the unique structure of oriC that allows the cell to initiate DNA replication correctly and at the proper time.Furthermore, it has been reported that the SeqA protein in bacterial cells, which represses DNA replication activity, promotes helical changes in DNA structure that cause positive supercoiling of the segment (38).
To support studies about bent DNA structure, atomic force microscopy has recently been performed in the M13 plasmid replication origin (39), providing independent evidence that this replication origin contains a stable bend.
The analysis of the 1892-bp fragment of the X. fastidiosa nucleotide sequence shows two or more adenine/ thymine tracts phased with the helical turn, located around the bent DNA sites.Similarly, the CAnT motif can also be found in DNA sequence-directed curvatures (40).Sequence analyses of the three bent sites revealed a predominance of stretches of multiple poly (dA) and poly (dT) tracts around the bent sites, showing a periodicity of ~10 bp or multiples of this value.It is also possible to observe five GATC motifs, two of which are located in the replication origin (oriC).It has been reported that the GATC motif also contributes to intrinsic DNA curvature at oriC, and the degree of bending is modulated by methylation (37).Furthermore, we also identified tracts of six nucleotides, named ATP-dependent DnaA box (32).
The results reported here show that the oriC of the related prokaryotes X. fastidiosa 9a5c and X. fastidiosa Temecula1 show great similarities in both their 2-D trajectories and helical parameters for curvature.In the other two bacterial oriC analyzed here, from B. subtilis and E. coli, both the value of the ENDS ratio peaks and the 2-D trajectory of the curvature increased.
The present study demonstrated that the X. fastidiosa 9a5c oriC has particular features such as intrinsic bent DNA sites which induce a curved DNA structure in this region.This structure is probably involved in the initiation of DNA replication for this organism.Furthermore, in silico analysis of three related bacterial oriC sequences showed similar negative roll angles, as well as twist values greater than 34.00°.A particular 2-D trajectory was observed for each replication initiation segment.

Figure 2 .
Figure 2. Electrophoretic mobility analysis of the Xylella fastidiosa oriC.The restriction map of the p16Kori clone is at the top.The R-value of 1.12 is shown above the fragment, which is indicated on the gels by white vertical arrows; black horizontal arrows indicate the plasmid pBluescript (pBS).M = molecular weight marker 1-kb Ladder; AGA = 1.0%agarose gel; PA and PA + EtBr = 6% polyacrylamide gels without and with ethidium bromide, respectively; B = BamHI; S = SmaI restriction sites.

Figure 3 .
Figure 3.In silico analysis of the Xylella fastidiosa 9a5c oriC chromosomal segment.The restriction map is at the top; it contains the rpmH gene initial sequence, the 141-bp intergenic region, the dnaA gene, the replication origin oriC, and the 5' end sequence of the dnaN gene.The arrows indicate the start and direction of genetic transcription.The intrinsic bent DNA sites at the 160-(b1), 860-(b2 ), and 1570-bp (b3 ) position are shown.The Map15a software, with 120-bp window width and a 10-bp step, was used to calculate the helical parameters ENDS ratio, ∆G, roll angle, and twist angle.

Figure 4 .
Figure 4.Figure 4.Figure 4.Figure 4.Figure 4. 2-D projection of the 3-D trajectory of the Xylella fastidiosa oriC chromosomal segment.The three intrinsic bent DNA sites, at the 160-(b1), 860-(b2), and 1570-bp (b3) positions, indicated by the of ENDS ratio (Figure 3) are shown.On the left side of the figure, rings of different sizes represent the free energy variation (∆G), which predicts the stability of the double helix.The larger gray rings represent higher ∆G values, and the small black rings represent lower values.The oriC replication origin is indicated by the presence of five DnaA boxes (R1-R5) and eight ACC repetition boxes of 24 nucleotides.The cube indicates the beginning of the sequence and the planned direction of the 2-D projection.The anticlockwise 30°a nd 60° rotation of these fragments, shown on the right side, confirms that the three bent DNA sites are important for the maintenance of the fragment shape.
Figure 4.Figure 4.Figure 4.Figure 4.Figure 4. 2-D projection of the 3-D trajectory of the Xylella fastidiosa oriC chromosomal segment.The three intrinsic bent DNA sites, at the 160-(b1), 860-(b2), and 1570-bp (b3) positions, indicated by the of ENDS ratio (Figure 3) are shown.On the left side of the figure, rings of different sizes represent the free energy variation (∆G), which predicts the stability of the double helix.The larger gray rings represent higher ∆G values, and the small black rings represent lower values.The oriC replication origin is indicated by the presence of five DnaA boxes (R1-R5) and eight ACC repetition boxes of 24 nucleotides.The cube indicates the beginning of the sequence and the planned direction of the 2-D projection.The anticlockwise 30°a nd 60° rotation of these fragments, shown on the right side, confirms that the three bent DNA sites are important for the maintenance of the fragment shape.
Figure 4.Figure 4.Figure 4.Figure 4.Figure 4. 2-D projection of the 3-D trajectory of the Xylella fastidiosa oriC chromosomal segment.The three intrinsic bent DNA sites, at the 160-(b1), 860-(b2), and 1570-bp (b3) positions, indicated by the of ENDS ratio (Figure 3) are shown.On the left side of the figure, rings of different sizes represent the free energy variation (∆G), which predicts the stability of the double helix.The larger gray rings represent higher ∆G values, and the small black rings represent lower values.The oriC replication origin is indicated by the presence of five DnaA boxes (R1-R5) and eight ACC repetition boxes of 24 nucleotides.The cube indicates the beginning of the sequence and the planned direction of the 2-D projection.The anticlockwise 30°a nd 60° rotation of these fragments, shown on the right side, confirms that the three bent DNA sites are important for the maintenance of the fragment shape.
Figure 4.Figure 4.Figure 4.Figure 4.Figure 4. 2-D projection of the 3-D trajectory of the Xylella fastidiosa oriC chromosomal segment.The three intrinsic bent DNA sites, at the 160-(b1), 860-(b2), and 1570-bp (b3) positions, indicated by the of ENDS ratio (Figure 3) are shown.On the left side of the figure, rings of different sizes represent the free energy variation (∆G), which predicts the stability of the double helix.The larger gray rings represent higher ∆G values, and the small black rings represent lower values.The oriC replication origin is indicated by the presence of five DnaA boxes (R1-R5) and eight ACC repetition boxes of 24 nucleotides.The cube indicates the beginning of the sequence and the planned direction of the 2-D projection.The anticlockwise 30°a nd 60° rotation of these fragments, shown on the right side, confirms that the three bent DNA sites are important for the maintenance of the fragment shape.

Figure 4 . 2 -
Figure 4.Figure 4.Figure 4.Figure 4.Figure 4. 2-D projection of the 3-D trajectory of the Xylella fastidiosa oriC chromosomal segment.The three intrinsic bent DNA sites, at the 160-(b1), 860-(b2), and 1570-bp (b3) positions, indicated by the of ENDS ratio (Figure 3) are shown.On the left side of the figure, rings of different sizes represent the free energy variation (∆G), which predicts the stability of the double helix.The larger gray rings represent higher ∆G values, and the small black rings represent lower values.The oriC replication origin is indicated by the presence of five DnaA boxes (R1-R5) and eight ACC repetition boxes of 24 nucleotides.The cube indicates the beginning of the sequence and the planned direction of the 2-D projection.The anticlockwise 30°a nd 60° rotation of these fragments, shown on the right side, confirms that the three bent DNA sites are important for the maintenance of the fragment shape.

Figure 5 .
Figure 5.Figure 5.Figure 5.Figure 5.Figure 5. Sequence analysis of the intrinsic bent DNA sites b1, b2, and b3.The nucleotides on the peaks of the bent DNA sites are within the rectangle.The initial sequence of the rpmH gene (105 bp in capital letters), an intergenic region of 141 bp (lower case letters), part of the dnaA gene, the replication origin segment oriC, and the initial sequence of the dnaN gene (24 bp in capital letters) are indicated.Two or more adenine/thymine tracts phased with the DNA helix turn are underlined.The CAnT motif, which can be observed in the center or around the curvature, is indicated by double underlining.Two tracts of 16 AT-rich nucleotides are indicated for the oriC (in bold).Motifs of the six nucleotide consensus sequence for the ATP-dependent DnaA box are represented by wavy lines, and the location and direction of the five DnaA boxes (R1-R5 in gray) are indicated.The ACC box with 24 nucleotides is in bold and underlined.The five GATC repetitions are in italic and bold.The oriC sequence starts 3 bp upstream of the center of the bent DNA site b3 (star).
Figure 5.Figure 5.Figure 5.Figure 5.Figure 5. Sequence analysis of the intrinsic bent DNA sites b1, b2, and b3.The nucleotides on the peaks of the bent DNA sites are within the rectangle.The initial sequence of the rpmH gene (105 bp in capital letters), an intergenic region of 141 bp (lower case letters), part of the dnaA gene, the replication origin segment oriC, and the initial sequence of the dnaN gene (24 bp in capital letters) are indicated.Two or more adenine/thymine tracts phased with the DNA helix turn are underlined.The CAnT motif, which can be observed in the center or around the curvature, is indicated by double underlining.Two tracts of 16 AT-rich nucleotides are indicated for the oriC (in bold).Motifs of the six nucleotide consensus sequence for the ATP-dependent DnaA box are represented by wavy lines, and the location and direction of the five DnaA boxes (R1-R5 in gray) are indicated.The ACC box with 24 nucleotides is in bold and underlined.The five GATC repetitions are in italic and bold.The oriC sequence starts 3 bp upstream of the center of the bent DNA site b3 (star).
Figure 5.Figure 5.Figure 5.Figure 5.Figure 5. Sequence analysis of the intrinsic bent DNA sites b1, b2, and b3.The nucleotides on the peaks of the bent DNA sites are within the rectangle.The initial sequence of the rpmH gene (105 bp in capital letters), an intergenic region of 141 bp (lower case letters), part of the dnaA gene, the replication origin segment oriC, and the initial sequence of the dnaN gene (24 bp in capital letters) are indicated.Two or more adenine/thymine tracts phased with the DNA helix turn are underlined.The CAnT motif, which can be observed in the center or around the curvature, is indicated by double underlining.Two tracts of 16 AT-rich nucleotides are indicated for the oriC (in bold).Motifs of the six nucleotide consensus sequence for the ATP-dependent DnaA box are represented by wavy lines, and the location and direction of the five DnaA boxes (R1-R5 in gray) are indicated.The ACC box with 24 nucleotides is in bold and underlined.The five GATC repetitions are in italic and bold.The oriC sequence starts 3 bp upstream of the center of the bent DNA site b3 (star).
Figure 5.Figure 5.Figure 5.Figure 5.Figure 5. Sequence analysis of the intrinsic bent DNA sites b1, b2, and b3.The nucleotides on the peaks of the bent DNA sites are within the rectangle.The initial sequence of the rpmH gene (105 bp in capital letters), an intergenic region of 141 bp (lower case letters), part of the dnaA gene, the replication origin segment oriC, and the initial sequence of the dnaN gene (24 bp in capital letters) are indicated.Two or more adenine/thymine tracts phased with the DNA helix turn are underlined.The CAnT motif, which can be observed in the center or around the curvature, is indicated by double underlining.Two tracts of 16 AT-rich nucleotides are indicated for the oriC (in bold).Motifs of the six nucleotide consensus sequence for the ATP-dependent DnaA box are represented by wavy lines, and the location and direction of the five DnaA boxes (R1-R5 in gray) are indicated.The ACC box with 24 nucleotides is in bold and underlined.The five GATC repetitions are in italic and bold.The oriC sequence starts 3 bp upstream of the center of the bent DNA site b3 (star).

Figure 5 .
Figure 5.Figure 5.Figure 5.Figure 5.Figure 5. Sequence analysis of the intrinsic bent DNA sites b1, b2, and b3.The nucleotides on the peaks of the bent DNA sites are within the rectangle.The initial sequence of the rpmH gene (105 bp in capital letters), an intergenic region of 141 bp (lower case letters), part of the dnaA gene, the replication origin segment oriC, and the initial sequence of the dnaN gene (24 bp in capital letters) are indicated.Two or more adenine/thymine tracts phased with the DNA helix turn are underlined.The CAnT motif, which can be observed in the center or around the curvature, is indicated by double underlining.Two tracts of 16 AT-rich nucleotides are indicated for the oriC (in bold).Motifs of the six nucleotide consensus sequence for the ATP-dependent DnaA box are represented by wavy lines, and the location and direction of the five DnaA boxes (R1-R5 in gray) are indicated.The ACC box with 24 nucleotides is in bold and underlined.The five GATC repetitions are in italic and bold.The oriC sequence starts 3 bp upstream of the center of the bent DNA site b3 (star).