Genetic Diversity of Pierce's Disease Strains and Other Pathotypes of Xylella fastidiosa

doi:10.1128/AEM.67.2.895-903.2001

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Applied and Environmental Microbiology, February 2001, p. 895-903, Vol. 67, No. 2
0099-2240/01/$04.00+0 DOI: 10.1128/AEM.67.2.895-903.2001
Copyright © 2001, American Society for Microbiology. All rights reserved.

Genetic Diversity of Pierce's Disease Strains and Other Pathotypes of Xylella fastidiosa

Mavis Hendson,¹^, Alexander H. Purcell,¹^,^* Deqiao Chen,¹ Chris Smart,²^, Magalie Guilhabert,² and Bruce Kirkpatrick²

Division of Insect Biology, University of California, Berkeley, California 94720-3112,¹ and Department of Plant Pathology, University of California, Davis, California 95616²

Received 22 May 2000/Accepted 5 December 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results Discussion References

Strains of Xylella fastidiosa isolated from grape, almond, maple, and oleander were characterized by enterobacterial repetitiveintergenic consensus sequence-, repetitive extragenic palindromicelement (REP)-, and random amplified polymorphic DNA (RAPD)-PCR;contour-clamped homogeneous electric field (CHEF) gel electrophoresis;plasmid content; and sequencing of the 16S-23S rRNA spacer region.Combining methods gave greater resolution of strain groupingsthan any single method. Strains isolated from grape with Pierce'sdisease (PD) from California, Florida, and Georgia showed greaterthan previously reported genetic variability, including plasmidcontents, but formed a cluster based on analysis of RAPD-PCR products,NotI and SpeI genomic DNA fingerprints, and 16S-23S rRNA spacerregion sequence. Two groupings of almond leaf scorch (ALS) strainswere distinguished by RAPD-PCR and CHEF gel electrophoresis, butsome ALS isolates were clustered within the PD group. RAPD-PCR,CHEF gel electrophoresis, and 16S-23S rRNA sequence analysis producedthe same groupings of strains, with RAPD-PCR resolving the greatestgenetic differences. Oleander strains, phony peach disease (PP),and oak leaf scorch (OLS) strains were distinct from other strains.DNA profiles constructed by REP-PCR analysis were the same orvery similar among all grape strains and most almond strains butdifferent among some almond strains and all other strains tested.Eight of 12 ALS strains and 4 of 14 PD strains of X. fastidiosaisolated in California contained plasmids. All oleander strainscarried the same-sized plasmid; all OLS strains carried the same-sizedplasmid. A plum leaf scald strain contained three plasmids, twoof which were the same sizes as those found in PP strains. Thesefindings support a division of X. fastidiosa at the subspeciesor pathovarlevel.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results Discussion References

Xylella fastidiosa (Wells et al.) (35) is a gram-negative, xylem-inhabiting bacterium that causes Pierce's disease (PD)of grape, phony peach disease (PP), periwinkle wilt, citrus variegatedchlorosis, and leaf scorch diseases of almond (almond leaf scorch[ALS]), plum (PLS), elm, maple, oak (OLS), and sycamore (16,27). All strains of X. fastidiosa are currently classified asone species but differ in important respects in plant host rangeand pathogenicity. The geographic isolation of the plant diseasescaused by X. fastidiosa restricts the easy comparison of the pathologicalcharacteristics of the various strains. Previous studies differentiatedX. fastidiosa strains on the basis of pathogenicity, nutritionalrequirements (16), DNA homology (19), structural protein analysis(3), restriction fragment length polymorphisms (RFLPs) (4),and random amplified polymorphic DNA (RAPD)-PCR (1, 6, 9,25, 27). RFLP and DNA-DNA hybridization studies revealed distinctdifferences between PD strains and strains that cause PP, PLS,and periwinkle wilt (4, 19). Pooler et al. (25) distinguishedfive groups of X. fastidiosa using RAPD-PCR: the citrus group,plum-elm group, grape-ragweed group, almond group, and mulberrygroup. Strains of X. fastidiosa causing OLS formed a separatecluster from PD strains (6).

The high levels of DNA homology (>85%) (35) among X. fastidiosa strains indicate that differences among strains would primarilylie in the linear arrangement of cistrons within the genome. Geneticanalyses using repetitive extragenic palindromic element (REP)-PCR,which utilizes conserved PCR primer sequences that reside withinrepetitive elements distributed throughout the prokaryote genome,have been widely used to identify and assess the genetic diversityof prokaryotes (34). Differences revealed by RAPD-PCR (36)and REP-PCR (34) have also been useful in characterizing differencesamong closely related strains (6, 25). Contour-clamped homogeneouselectric field (CHEF) electrophoresis (7) allows the separationof large DNA molecules by electrophoresis. By digesting the genomewith enzymes which cut infrequently, DNA fingerprints which consistof a comparatively small number (generally fewer than 30 bands)of large fragments can be generated. Fewer fragments allow easiercomparison of strains than the hundreds of fragments that aretypically produced using conventional restriction enzyme digestion.Significant sequence heterogeneity within the 16S-23S rRNA spacerregion of Proteobacteria has been used to discriminate betweendifferent species of Proteobacteria and to detect heterogeneitywithin species (2, 18), but closely related microorganismsoften have very similar spacer regions. RAPD analysis distinguishedcoffee strains from citrus strains of X. fastidiosa (9, 29).Plasmids have been found in some strains of X. fastidiosa (4,24) but have not been extensivelystudied.

The objective of this study was to analyze the genetic relatedness of X. fastidiosa strains in California that were isolatedfrom grape, almond, and oleander. For comparison, strains of X.fastidiosa which cause PD, PP, PLS, and OLS isolated from thesoutheastern United States were also characterized. X. fastidiosastrains were analyzed by RAPD-PCR (36), REP-PCR (34), CHEFelectrophoresis (7, 8) of genomic DNA digested with rare-cuttingrestriction enzymes, 16S-23S rRNA spacer sequences, and plasmidcontent.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results Discussion References

Strains tested. Forty-six strains of X. fastidiosa that were analyzed in this study are listed in Table 1. In addition, we analyzed over80 other strains isolated from grapevines from widespread regionsof California by REP-and enterobacterial repetitive intergenicconsensus sequence (ERIC)-PCR. Each strain was isolated from theindicated host plants (Table 1) with disease symptoms. All strainswere grown by plating 100 µl of 10¹⁰-CFU/ml culture on PW agar medium (10) or the modified PWG medium(15) and incubating at 28°C for 7 to 10 days.

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TABLE 1. Strains of X. fastidiosa used in this study

DNA extraction for PCR. Bacterial DNA was extracted using the CTAB minipreparation method described by Wilson (37). Aerosol-resistant tips wereused in procedures for the extraction of DNA that was used inPCRs.

PCR conditions and primers. In PCRs for the specific detection of X. fastidiosa strains, primers RST31 (5'-GCGTTAATTTTCGAAGTGATTCGATTGC-3') and RST33(5'-CACCATTCGTATCCCGGTG-3') were used as described by Minsavageet al. (21).

RAPD-PCRs were performed using 10-base primers (Kit AA; Operon Technologies, Inc., Alameda, Calif.). Amplifications were performedin a 25-µl reaction volume containing 25 ng of genomic DNA; 25pmol of a single primer; 2 mM MgCl₂; 100 µM (each) dATP, dCTP,dGTP, and dTTP; 10 mM Tris HCl [pH 9]; 50 mM KCl; 0.1% TritonX-100; and 0.5 U of Amplitaq DNA polymerase (Perkin-Elmer, FosterCity, Calif.). RAPD-PCRs were done with a DNA Thermal Cycler (Perkin-Elmer)using 1 cycle of 1 min at 94°C; 45 cycles of 1 min at 94°C, 1min at 34°C, and 2 min at 72°C; and a final extension of 10 minat 72°C.

Eighty X. fastidiosa grape strains that were isolated from separate grapevines showing typical symptoms of Pierce's diseasewere analyzed by ERIC- and REP-PCR. A subset of strains shownin Table 1 was also analyzed by ERIC-PCR. Individual coloniesgrowing on PW agar medium were transferred directly into the REP-PCRmixture, as previously described by Opgenorth et al. (23). PCRconditions using ERIC- and REP-PCR primers and agarose gel electrophoresisconditions of the PCR products were the same as described by Opgenorthet al. (23). Similarities and differences among the strainswere comparedqualitatively.

The 16S-23S rRNA intergenic spacer regions of X. fastidiosa strains were PCR amplified using primers G1 and L1, which arelocated in highly conserved regions within the 16S and 23S rRNAgenes, respectively (18). Primer G1 (5'-GAAGTCGTAACAAGG-3')is located at the 3' end of the 16S rRNA gene 30 to 40 nucleotidesupstream of the spacer region, and L1 (5'-CAAGGCATCCACCGT-3')is located at the 5' end of the 23S rRNA gene, approximately 20bases downstream from the spacer region. PCR mixtures contained25 ng of genomic DNA; 25 pmol of G1; 25 pmol of L1; 10 mM Tris[pH 8.0]; 50 mM KCl; 2.5 mM MgCl₂; 200 µM (each) dATP, dCTP, dGTP,and dTTP, and 0.5 U of Amplitaq DNA polymerase (Perkin-Elmer).A DNA Thermal Cycler (Perkin-Elmer) was used, with 1 cycle of5 min at 94°C; 35 cycles of 94°C for 40 s, 55°C for 1 min, and72°C for 2 min; and a final extension of 10 min at 72°C.

Except for REP-PCR products, gel electrophoresis of PCR amplification products was performed with 1.4% agarose gels in TAEbuffer (20) at 3.5 V/cm. After the gels were stained with ethidiumbromide (0.5 µg/ml), PCR products were visualized on a UV transilluminatorandphotographed.

Sequencing of the 16S-23S rRNA intergenic spacer region. PCR-amplified intergenic spacer regions were purified using Ultrafree tubes (Millipore, Bedford, Mass.). Both strands of thespacer regions were sequenced by the dideoxy chain terminationmethod (30) using a cycle-sequencing format (Perkin-Elmer AppliedBiosystems, Foster City, Calif.). Sequencing reaction mixtureswere electrophoresed, and nucleotide sequences were recorded usingthe ABI 377 automated sequencer (Perkin-Elmer Applied Biosystems).Phylogenetic analysis of the 16S-23S rRNA sequences was resolvedusing the PAUP Software program, version 3.1 (33).

Analysis of RAPD-PCR product profiles. RAPD-PCR product profiles of all isolates were compared, and the similarities of PCR products between pairs of strains werescored with the Jaccard similarity coefficient (32). The Jaccardcoefficient, S, is the proportion of shared DNA fragments in twoisolates and is calculated with the formula S = 2n_xy/(n_x + n_y),where n_x is the total number of fragments in isolate x, n_y isthe total number in isolate y, and n_xy is the number of fragmentscommon to the two isolates. The distance (d) between two strainsis calculated with the formula d = 1 $-$ S. A d value of 0 indicatesthat the two isolates have identical RAPD-PCR products, and avalue of 1.0 indicates that the two isolates have no PCR productsin common. A distance matrix of pairwise comparison between strainswas constructed. The relationship between strains was analyzedwith the neighbor-joining program of PHYLIP (12).

CHEF gel electrophoresis. DNA for CHEF electrophoresis was prepared by a modification of the method of Cooksey and Graham (8). Cells grown on plateswere harvested and washed with SE buffer (75 mM NaCl; 25 mM EDTA[pH 7.5]), and the cell density was adjusted to 10⁹ CFU/ml in SE buffer. A 0.5-ml sample of the bacterial suspensionwas mixed with 0.5 ml of 2% agarose (pulse-field certified; Bio-Rad,Richmond, Calif.) in 10 mM Tris, 10 mM MgCl₂, and 0.1 mM EDTA(pH 7.5). Plugs were cast in plug molds (1 by 0.5 cm; Bio-Rad)and placed at 4°C for 5 min to allow the agarose to solidify.Ten plugs were placed in 5 ml of lysis solution consisting ofproteinase K (0.5 mg/ml; Bethesda Research Laboratories, Gaithersburg,Md.), 1% N-lauroylsarcosine, and 0.5 M EDTA (pH 9.5). After overnightincubation at 50°C, the plugs were washed four times with 20 mMTris (pH 8.0) and 50 mM EDTA, 1 h each time, at room temperaturewith gentle agitation. In the second wash, 1 mM phenylmethylsulfonylfluoride (Sigma, St. Louis, Mo.) was added to inactivate the residualproteinase K. Plugs were then washed five times with TE (10 mMTris, 10 mM EDTA, [pH 8.0]), 10 min for each wash, with gentleagitation at room temperature. The genomic DNA immobilized inthe plugs was incubated with the appropriate restriction bufferat room temperature for 1 h prior to the addition of the restrictionenzyme. Digestions were carried out overnight at 37°C in 1× restrictionbuffer, 1 mg of bovine serum albumin per ml, and one of the followingenzymes: NheI (10 U), NotI (10 U), SacII (10 U), SpeI (6 U), orXbaI (6 U) (New England Biolabs, Beverly, Mass.). Agarose gelelectrophoresis of digested DNA fragments was performed with a1% agarose gel (13 by 14 cm) using 0.5× TBE buffer (20). One-thirdof the agarose plug was inserted into each well in the gel. Wellsin the gel were filled with agarose to seal the wells. Agaroseplugs containing concatemers of $lambda$ DNA (Bio-Rad) were used as molecularsize standards. Electrophoresis was carried out with 0.5× TBEat 14°C for 20 h at 6 V/cm with a 1- to 12-s switch time rampat an included angle of 120° using a CHEF-DR III pulsed-fieldelectrophoresis system (Bio-Rad). After electrophoresis, the gelwas stained in 0.5 µg of ethidium bromide per ml for 30 min. DNAwas visualized and photographed as describedabove.

The similarities in restriction fragment length patterns generated by CHEF electrophoresis between pairs of strains were scoredwith the Jaccard coefficient as described above. A distance matrixwas obtained by pairwise comparison between strains. The relatednessof strains was determined by neighbor-joining analysis using thePHYLIP computer package (12).

Plasmid isolation and analysis. Strains of X. fastidiosa were grown by plating 100 µl of 10¹⁰ CFU/ml culture on PWG medium and incubation at 28°C for 7 days.Cells from one plate were resuspended in 1 ml of TE buffer, washedonce in TE buffer, and finally resuspended in 100 µl of TE buffer.Plasmids were isolated by the alkaline minipreparation method(20). Plasmid DNA was resuspended in 10 µl of TE buffer. Fivemicroliters of native plasmid DNA was electrophoresed to determinethe number of plasmids present in the strains. Total plasmid DNAin the remaining 5 µl was digested with HindIII by standard procedures(20), and the resulting fragments were analyzed by agarose gelelectrophoresis with TAE buffer (20).

	RESULTS

Top Abstract Introduction Materials and Methods Results Discussion References

Analysis of PCR products using primers specific for X. fastidiosa. All strains gave the same-sized PCR product (0.75 kb) (results not shown) in reactions using primers RST31 and RST33. PCRproducts of X. fastidiosa strains isolated from oak, oleander,peach, and plum and all ALS strains excluding ALS1, Manteca, andTulare were digested into two fragments of approximately 0.55and 0.2 kb using RsaI (results not illustrated). In contrast,the 0.75-kb PCR products from the three ALS strains, all PD strains,and the strain isolated from maple were not digested with RsaI.

Sequence analysis of the 16S-23S rRNA intergenic spacer region. A region of approximately 500 bases containing the 16S-23S rRNA intergenic spacer region of all strains listed in Table 1was sequenced. The intergenic spacer region of all X. fastidiosastrains contained tRNAs for alanine (positions 133 to 191) andisoleucine (positions 225 to 272). Analysis of this region revealedfour groupings of strains: (i) most almond strains, all peachstrains, and the plum strain, (ii) oak strains, (iii) oleanderstrains, and (iv) grape strains, a few almond strains, and themaple strain. With the exception of almond strains ALS1, Manteca,and Tulare, all strains of X. fastidiosa isolated from the samehost had identical sequences within the 16S-23S rRNA region. StrainsALS1, Manteca, and Tulare and the strain isolated from maple hadthe same sequence as strains isolated from grape. Strains isolatedfrom grape and maple and almond strains ALS1, Manteca, and Tularediffered from the other strains at positions 56 and 485. The sequenceof strains isolated from oleander (28) was distinguished fromall other strains at two base positions (213 and 328). Strainsof X. fastidiosa isolated from oak differed from all other strainsat position 351. The 16S-23S sequences of strains isolated fromalmond (except for ALS1, Manteca, and Tulare), plum, and peachwere identical and differed from other strains at positions 327,337, 408, 419, and431.

ERIC- and REP-PCR fingerprinting of X. fastidiosa strains. Grape strains of X. fastidiosa from plants from the southeastern United States had the same ERIC-PCR profiles as grape strainsfrom California (Fig. 1, lanes 1 to 5). All 80 strains from widelydistributed locations in California had the same ERIC- and REP-PCRprofiles (data not shown). The same profile was also observedin a California isolate from maple exhibiting widespread leafscorching and one of the almond strains (ALS1). Two other almondstrains (ALS2 and ALS3) were identical to each other but possessedthree or four DNA bands differing from those in the grape strains.The two oak strains from the southeastern United States were similarto each other and different from all the other strains. Similarly,the oleander strains were identical to each other but differentfrom the other strains. Despite numerous attempts, we were notable to amplify an ERIC-PCR profile from either the plum or peachstrains from the southeastern United States.

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FIG. 1. REP-PCR analysis of X. fastidiosa strains. ERIC-PCR profiles of X. fastidiosa strains from diverse plant hosts or geographical locations are shown. Lane 1, grape isolate from Georgia (strain R116V3); lane 2, grape from Florida (PD95-2); lane 3, grape from California (Stags Leap); lane 4, maple from California; lane 5, grape from California (Conn Creek); lane 6, almond (ALS1); lane 7, almond (ALS2); lane 8, almond (ALS3); lane 9, 1-kb size standard; lane 10, oak from Florida (88-9); lane 11, oak from Georgia (OLS#2); lane 12, oleander (Ann1); lane 13, oleander (TR1); lane 14, water control.

RAPD-PCR analysis. Of the 20 individual 10-base oligomers used as primers in RAPD-PCR analysis of X. fastidiosa strains listed in Table 1, 4primers (OP-AA-05, OP-AA-15, OP-AA-18, and OP-AA-19) yielded noPCR product. Six primers (OP-AA-07, OP-AA-13, OP-AA-14, OP-AA-16,OP-AA-17, and OP-AA-19) yielded one or two PCR products (resultsnot shown) that were uniform among all strains tested. Ten primers(OP-AA-01, OP-AA-02, OP-AA-03, OP-AA-04, OP-AA-06, OP-AA-08, OP-AA-09,OP-AA-10, OP-AA-11, and OP-AA-12) yielded complex RAPD fingerprintsthat allowed the distinction of strains isolated from differenthosts. The PCR products of selected strains using primer OP-AA-01are shown in Fig. 1. PCR products of all strains were compared,and a distance matrix was constructed. A dendrogram produced bythe neighbor-joining algorithm of the phylogeny inference package,PHYLIP, is shown (see Fig. 3). As depicted in Fig. 2 and 3, allstrains of X. fastidiosa causing PD were similar to ALS strainsALS1, Manteca, and Tulare. This included PD strains from California,Florida, and Georgia. Strains causing ALS were further dividedinto second and third groupings; the latter consisted of strainsALS6 and Contra Costa (Fig. 2 and 3). Strains isolated from oleander,oak, peach, and plum each formed separate clusters. Strains ofX. fastidiosa isolated from the plum and peach clusters were moresimilar to OLS strains than to other groupings (Fig. 2 and 3).

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FIG. 2. Agarose gel electrophoresis of RAPD-PCR products (primer OP-AA-01) synthesized using the template DNA of various strains. Lane 1, 1-kb ladder; lane 2, strain ALS2; lane 3, ALS3; lane 4, ALS4; lane 5, ALS5; lane 6, ALS7; lane 7, ALS9; lane 8, Dixon; lane 9, ALS6; lane 10, Contra Costa; lane 11, ALS1; lane 12, Manteca; lane 13, Tulare; lane 14, Conn Creek; lane 15, Douglas; lane 16, Hopland; lane 17, Medeiros; lane 18, Meyley; lane 19, Moore Park; lane 20, Oxford; lane 21, 1-kb ladder; lane 22, Santa Cruz; lane 23, Traver; lane 24, UCLA; lane 25, 95-2; lane 26, 95-4; lane 27, 95-9; lane 28, R116V3; lane 29, R118V3-4; lane 30, Maple; lane 31, T1c; lane 32, TR1; lane 33, Plum 2#4; lane 34, 4S3; lane 35, 5R1; lane 36, 5S2; lane 37, Oak 88-9; lane 38, Oak 92-3; lane 39, Oak 92-10; lane 40, Stucky.

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FIG. 3. Phylogram based on distance data obtained by RAPD-PCR analysis. A distance matrix was constructed by pairwise comparison of the RAPD PCR products among strains. The Jaccard similarity coefficient (32) was used (S = 2n_xy/n_x + n_y), where n_xy is the number of PCR products common to strains x and y, n_x is the number of bands present in strain x, and n_y is the number of bands present in strain y. The scale bar indicates relative dissimilarity between strains. A, almond; G, grape; M, maple; O, oak; Ol, oleander; P, peach; Pl, plum.

CHEF electrophoresis of genomic DNA. Restriction fragments of genomic DNA of X. fastidiosa strains produced by digestion with enzymes NheI, SacII, and XbaI wereless than 50 kb in size and too numerous to make good comparisonsbetween strains. Fragments of genomic DNA digested with NotI andSpeI were generally larger than 50 kb and proved to be usefulfor comparing strains. Figure 4 shows a CHEF gel of DNAs fromrepresentative X. fastidiosa strains digested by NotI and SpeI.The groupings based on SpeI digestion of genomic DNA correspondedto groupings established by NotI digestion of genomic DNA.

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FIG. 4. CHEF-agarose gel electrophoresis of the genomic DNA of various strains digested with enzyme NotI digests. Lane 1, one concatemer; lane 2, UCLA; lane 3, Douglas; lane 4, 95-4; lane 5, R118V3-4; lane 6, ALS1; lane 7, Manteca; lane 8, Maple; lane 9, ALS2; lane 10, ALS3; lane 11, ALS5; lane 12, ALS6; lane 13, 5S2; lane 14, 5R1; lane 15, Plum 2#4; lane 16, Oak 92-3; lane 17, Stucky; lane 18, Ann1; lane 19, TR1; lane 20, one concatemer.

In general, CHEF and RFLP patterns of strains isolated from the same plant host were similar or identical (Fig. 4). The exceptionswere the almond strains ALS1, Manteca, and Tulare, which had fingerprintssimilar to those of strains isolated from grape from California,Florida, and Georgia and of the strain isolated from maple. Thesegroupings agreed with those established by ERIC-PCR fingerprinting.Thus, almond strains formed three distinct RFLP groups. Group1 included strains ALS1, Manteca, and Tulare, which had restrictionfingerprints that were similar to those of grape strains. Thesecond RFLP group consisted of strains ALS2, ALS3, ALS4, ALS5,ALS7, ALS9, and Dixon. The third group, consisting of strainsALS6 and Contra Costa, differed from strains of almond groups1 and 2. A distance matrix constructed by pairwise comparisonof restriction fragments among strains with the Jaccard coefficientand analyzed by neighbor-joining analysis resulted in the treeshown in Fig. 5. Groupings of strains elucidated by CHEF electrophoresisagreed with groupings established by REP- and RAPD-PCR analysis.

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FIG. 5. Phylogram based on distance data obtained by CHEF-gel electrophoresis of NotI- and SpeI-restricted genomic DNA. A distance matrix was constructed by pairwise comparison of the RAPD-PCR products among strains. The Jaccard similarity coefficient (32) was used. The scale bar indicates relative dissimilarity between strains. A, almond; G, grape; M, maple; O, oak; Ol, oleander; P, peach; and Pl, plum.

Plasmid analysis. Plasmids were detected in 27 of 44 strains tested. Native plasmid DNA was electrophoresed to determine the number of plasmidsin the 27 strains (results not shown; Table 2). When total plasmidDNA was digested with HindIII, nine different RFLP patterns (Fig.6; Table 2) were observed. Figure 6 shows HindIII digests ofthe various plasmids observed among the X. fastidiosa strainstested. HindIII-digested plasmid DNAs of all OLS strains (Stucky,OLS#2, Oak 88-9, Oak 92-3, and Oak 92-10) were identical (plasmidprofile B, Table 2). The same plasmid profile was observed inall oleander leaf scorch strains (Ann1, PF1, TR1, and T1c) (plasmidprofile H). The strain causing PLS contained three plasmids (resultsnot shown; plasmid profiles E, F, and G), two of which appearedto have the same HindIII patterns as the plasmids isolated fromPP strains 5S3 and 5R1 (plasmid profiles E and F). Peach strain4S3 was not evaluated for plasmid content. ALS strains ALS1 andALS3 did not harbor any plasmids. The restriction profile of theplasmid present in strain ALS6 (plasmid I profile) differed fromthat found in other almond strains. Contra Costa (almond group3) contained no plasmids, whereas ALS6 (almond group 3) containedone plasmid. ALS strains Dixon, Tulare, ALS2, ALS4, ALS5, ALS7,and ALS9 and PD strains Medeiros, Moore Park, and Traver carriedthe same plasmid (plasmid profile A). Strain UCLA contained fourplasmids (results not shown; plasmid profiles J through M). HindIIIdigestion of plasmid DNA isolated from strain UCLA indicated thata subset of the fragments were the same size as those found inplasmid profile A. The HindIII profiles of plasmid DNA of Floridagrape strains 95-2 and 95-10 were identical (plasmid profile C).The restriction pattern of the plasmid present in strain 95-4differed from those found in 95-2 and 95-10 (plasmid profile D).

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TABLE 2. Plasmids found among strains of X. fastidiosa^a

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FIG. 6. Agarose gel electrophoresis of HindIII-digested plasmid DNA from various X. fastidiosa strains. Lane 1, 1-kb ladder; lane 2, strain UCLA; lane 3, Tulare; lane 4, ALS4; lane 5, ALS6; lane 6, 95-2; lane 7, 95-4; lane 8, peach; lane 9, Plum 2#4; lane 10, Oak 88-9; lane 11, Ann1; lane 12, 1-kb ladder.

	DISCUSSION

Top Abstract Introduction Materials and Methods Results Discussion References

All of the methods of genetic analysis used in this study produced the same host-associated groupings of X. fastidiosa strains,but RAPD and CHEF methods distinguished the greatest degree ofgenetic heterogeneity. The 16S-23S spacer region sequences distinguishedfour major groups: (i) 9 of 12 almond strains, plum strains, andall peach strains; (ii) oak strains; (iii) oleander strains; and(iv) all grape strains, a maple strain, and 3 almond strains.REP-PCR and RAPD analyses delineated five groups by distinguishingalmond strains from peach and plum strains from the above fourgroups and separating almond strains into two groups: one withinthe grape group and another almond strain group distinct fromgrape. CHEF analysis identified the same five groups as did REP-PCRand RAPD analyses but revealed greater differences between grapeand almond strains. CHEF analysis identified six groupings amongthe strains studied by distinguishing differences in groupingsamong most almond strains; however, CHEF analysis gave less resolutionof genetic heterogeneity than RAPDanalysis.

ALS and PD are thought to be caused by the same or similar strains of X. fastidiosa (11, 22), but anomalies have beennoted. For example, in southern central California, ALS was absentfrom almond orchards that were adjacent to vineyards with a highincidence of PD (26). The reverse situation was noted in northerncentral California, where the incidence of PD was low in vineyardsthat were adjacent to almond orchards with a very high incidenceof ALS (26). Our results suggest that some almond strains (e.g.,ALS1, Manteca, and Tulare) may cause either PD or ALS under naturalconditions, but other strains (almond groups 2 and 3) probablycause disease mostly in field-grown almonds. Unlike oak, oleander,peach, and plum groups, which appear to be genetically uniform,ALS strains (groups 1, 2, and 3) differ considerably from eachother in REP- and RAPD-PCR and genomic DNA restriction fingerprints.However, strains from both distinctive groups of ALS strains producedALS symptoms after mechanical inoculation (R. P. Almeida and A.H. Purcell, unpublished data). It would be interesting to determinewhether the three groups of ALS strains differ in virulence inalmond andgrape.

Strains that cause PD or alfalfa dwarf disease under greenhouse conditions occur naturally among an unusually broad rangeof host plants (13, 17). Hewitt (14) speculated that thePD pathogen was introduced into California via the importationof plants (such as wild grapes used for grape rootstocks) fromsoutheastern North America, where PD is endemic. The similarityof RAPD-PCR products and genomic DNA restriction patterns amongPD strains from California, Florida, and Georgia supports thishypothesis. Grape isolates from California were genetically uniformwhen both ERIC and REP-PCR primers were used. Because REP-PCRanalyzes the distribution of repetitive sequences in bacterialgenomes, it is less likely to detect minor genetic changes thatcan be detected using select RAPD primers. The results obtainedwith REP-PCR suggest that California PD strains form a coherentcluster compared to Xylella strains that infect other woody plantspecies growing in diverse geographicalareas.

The genetic variation among PD strains of X. fastidiosa strains revealed by RAPD-PCR suggests either that these differencesamong PD strains have evolved over the past 130-plus years orthat genetically different strains were introduced into the stateor that some PD strains are indigenous to western North America.Among the California PD strains that were analyzed by RAPD-PCR,the north coastal strains (found in Alameda, Napa, Santa Cruz,and Sonoma counties) were more similar to each other than to southernCalifornia strains (found in Ventura, San Luis Obispo, and LosAngeles counties) or to central California strains (found in Fresno,Tulare, and Contra Costa counties) (Table 1). Additional strainswill have to be analyzed to determine if these putative geographicalgroupings consistently occur in these regions of California. Alternatively,some of the differences that were revealed by RAPD analyses couldbe due to the presence of extrachromosomal DNA, although therewas no consistent association between a particular RAPD patternand the presence or absence of plasmidDNA.

In contrast to the results reported by Chen et al. (4), we found plasmids in most of the X. fastidiosa strains analyzed.It is interesting to note that, although grape strains from theeast and west coasts of the United States have similar chromosomalDNA, they differed in plasmid DNA content. Furthermore, the sameplasmid profile (plasmid profile A) was common to both CalifornianPD and ALS strains whose chromosomal DNAs were genetically different,suggesting that this plasmid might be transferable between almondand grapestrains.

All of the molecular genetic analyses indicate that the strains of X. fastidiosa causing oleander leaf scorch (28) are distinctfrom PD, ALS, OLS, PP, and PLS strains. We did not detect anygenetic differences among the four oleander strains we examined.Oleander leaf scorch was observed in California in the mid-1990s,and the origin of the oleander leaf scorch strains is unknown.Our results best support the hypothesis that the current outbreakof oleander disease is the result of a single introduction orlimited number of introductions of a genetically uniform X. fastidiosastrain. Additional oleander strains will have to be analyzed inorder to substantiate thishypothesis.

The low variability of 16S-23S rRNA intergenic spacer region sequences among all X. fastidiosa strains tested indicates thatthey are phylogenetically closely related. CHEF electrophoresisof large genomic restriction fragments, REP- and RAPD-PCR products,and RsaI restriction of the genomic region specific to X. fastidiosaand flanked by oligonucleotide primers RST 31 and 33 (21) groupedoleander leaf scorch strains with ALS, OLS, PP, and PLS strains.But the sequence of the 16S-23S rRNA spacer region suggests thatoleander leaf scorch strains are more closely related to PD strains.This implies potential independent evolution of these particulargeneticloci.

RFLP studies by Chen et al. (4) indicated that strains of PD, ALS, and alfalfa dwarf disease comprise a PD RFLP group.The PLS cluster was distantly related to the Pierce's diseasegroup. Our results show that most ALS strains differ from PD strainsand that the plum group is closer to the almond group than tothe PDgroup.

If our results are supported by additional DNA-DNA hybridization analyses, these genetic groups of X. fastidiosa may representdistinct species. The availability of a complete sequence froma citrus variegated chlorosis strain (31) and several otherX. fastidiosa strains in the near future (http: //www.jgi.doe.gov/tempweb/jgi_microbial/html/index.html)should further clarify species differences among strains of Xylella.At the least, our findings support the suggestion of other groups(6, 9, 19, 24, 29) that X. fastidiosa should be taxonomicallydifferentiated at the subspecies or pathovar level. However, theabilities of various strains to infect and cause disease in thevarious plant host need to be examined before pathovars can bedesignated.

	ACKNOWLEDGMENTS

This work was supported by grants from the Napa Valley Pierce's Disease Task Force and the American VineyardFoundation.

We thank Stuart Saunders for help in maintaining cultures and other technicalassistance.

	FOOTNOTES

^* Corresponding author. Mailing address: Division of Insect Biology, 201 Wellman Hall, University of California, Berkeley, CA94720-3112. Phone: (510) 642-7285. Fax: (510) 642-7428. E-mail:purcell{at}nature.berkeley.edu.

Present address: Department of Justice, Berkeley, CA94710.

Present address: Department of Plant Pathology, Cornell University, Ithaca, NY14853.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results
Discussion
References

1. Banks, D., R. Albibi, J. Chen, O. Lamikanra, R. L. Jarret, and B. J. Smith. 1999. Specific detection of Xylella fastidiosa Pierce's disease strains. Curr. Microbiol. 39:85-88[CrossRef][Medline].

2. Barry, T., G. Colleran, M. Glennon, L. K. Dunican, and F. Gannon. 1991. The 16S/23S ribosomal spacer region as a target for DNA probes to identify eubacteria. PCR Methods Appl. 1:233-236.

3. Chang, C. J., and N. W. Schaad. 1982. Electrophoretic protein profiles of total cell envelopes of xylem-limited plant pathogenic rickettsia-like bacteria (RLB). Phytopathology 72:935-936.

4. Chen, J., C. J. Chang, and R. L. Jarret. 1992. Plasmids from Xylella fastidiosa. Can. J. Microbiol. 38:993-995.

5. Chen, J., C. J. Chang, R. L. Jarret, and N. Gawel. 1992. Genetic variation among Xylella fastidiosa strains. Phytopathology 82:973-977.

6. Chen, J., O. Lamikanra, C. J. Chang, and D. L. Hopkins. 1995. Randomly amplified polymorphic DNA analysis of Xylella fastidiosa Pierce's disease and oak leaf scorch pathotypes. Appl. Environ. Microbiol. 61:1688-1690[Abstract].

7. Chu, G., D. Vollrath, and R. W. Davis. 1986. Separation of large DNA molecules by contour-clamped homogeneous electric fields. Science 234:1582-1585[Abstract/Free Full Text].

8. Cooksey, D. A., and J. H. Graham. 1989. Genomic fingerprinting of two pathovars of phytopathogenic bacteria by rare-cutting restriction enzymes and field inversion gel electrophoresis. Phytopathology 79:745-750.

9. da Costa, P. I., C. F. Franco, V. S. Miranda, D. C. Teixeira, and J. S. Hartung. 2000. Strains of Xylella fastidiosa rapidly distinguished by arbitrarily primed PCR. Curr. Microbiol. 40:279-282[CrossRef][Medline].

10. Davis, M. J., W. J. French, and N. W. Schaad. 1981. Axenic culture of the bacteria associated with phony peach disease and plum leaf scald. Curr. Microbiol. 6:309-314[CrossRef].

11. Davis, M. J., S. W. Thompson, and A. H. Purcell. 1979. Etiological role of the xylem-limited bacterium causing Pierce's disease in almond leaf scorch. Phytopathology 70:472-475.

12. Felsenstein, J. 1993. PHYLIP (phylogeny inference package) version 3.5c. Department of Genetics, University of Washington, Seattle, Wash.

13. Freitag, J. H. 1951. Host range of the Pierce's disease virus of grapes as determined by insect transmission. Phytopathology 41:920-934.

14. Hewitt, W. B. 1958. The probable home of Pierce's disease virus. Plant Dis. Rep. 42:211-215.

15. Hill, B. L., and A. H. Purcell. 1995. Acquisition and retention of Xylella fastidiosa by an efficient vector, Graphocephala atropunctata. Phytopathology 85:209-212.

16. Hopkins, D. L. 1989. Xylella fastidiosa: xylem-limited bacterial pathogen of plants. Annu. Rev. Phytopathol. 27:271-290[CrossRef].

17. Hopkins, D. L., and W. C. Adlerz. 1988. Natural hosts of Xylella fastidiosa in Florida. Plant Dis. 72:429-431.

18. Jensen, M. A., J. A. Webster, and N. Straus. 1993. Rapid identification of bacteria on the basis of polymerase chain reaction-amplified ribosomal DNA spacer polymorphisms. Appl. Environ. Microbiol. 59:945-952[Abstract/Free Full Text].

19. Kamper, S. M., W. J. French, and S. R. DeKloet. 1985. Genetic relationships of some fastidious xylem-limited bacteria. Int. J. Syst. Bacteriol. 35:185-188.

20. Maniatis, T., E. F. Fritsch, and J. Sambrook. 1982. Molecular cloning $---$ a laboratory manual, p. 368-369. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.

21. Minsavage, G. V., C. M. Thompson, D. L. Hopkins, R. M. V. B. C. Leite, and R. E. Stall. 1994. Development of a polymerase chain reaction protocol for detection of Xylella fastidiosa in plant tissue. Phytopathology 84:456-461[CrossRef].

22. Mircetich, S. M., S. L. Lowe, W. J. Moller, and G. Nyland. 1976. Etiology of almond leaf scorch disease and transmission of the casual agent. Phytopathology 66:17-24.

23. Opgenorth, D. C., C. D. Smart, F. J. Louws, F. J. deBruijn, and B. C. Kirkpatrick. 1996. Identification of Xanthomonas fragariae field isolates by rep-PCR genomic fingerprinting. Plant Dis. 80:868-873.

24. Pooler, M. R., and J. S. Hartung. 1997. Sequence analysis of a 1296-nucleotide plasmid from Xylella fastidiosa. FEMS Microbiol. Lett. 155:217-222[CrossRef][Medline].

25. Pooler, M. R., J. S. Hartung, and R. G. Fenton. 1995. Genetic relationships among strains of Xylella fastidiosa from RAPD-PCR data. Curr. Microbiol. 31:134-137[CrossRef][Medline].

26. Purcell, A. H. 1980. Almond leaf scorch: leafhopper and spittle bug vectors. J. Econ. Entomol. 73:834-838.

27. Purcell, A. H. 1997. Xylella fastidiosa, a regional problem or global threat? J. Plant Pathol. 79:99-105.

28. Purcell, A. H., S. R. Saunders, M. Hendson, M. E. Grebus, and M. J. Henry. 1999. Causal role of Xylella fastidiosa in oleander leaf scorch. Phytopathology 89:53-58[CrossRef].

29. Rosato, Y. E., J. R. Neto, V. S. Miranda, E. F. Carlos, and G. P. Manfio. 1998. Diversity of a Xylella fastidiosa population isolated from Citrus sinensis affected by citrus variegated chlorosis in Brazil. Syst. Appl. Microbiol. 21:593-598.

30. Sanger, F., S. Nicklen, and A. R. Coulson. 1977. DNA sequencing with chain termination inhibitors. Proc. Natl. Acad. Sci. USA 74:5463-5467[Abstract/Free Full Text].

31. Simpson, A. A. J. G., F. C. Reinach, P. Arruda, F. A. Abreu, M. Acencio, R. Alvarenga, L. M. Alves, J. E. Araya, G. S. Baia, C. S. Baptista, et al. 2000. The genome sequence of the plant pathogen Xylella fastidiosa. Nature 406:151-157[CrossRef][Medline].

32. Sneath, P. H. A., and R. R. Sokal. 1973. Numerical taxonomy. W. H. Freeman and Co., San Francisco, Calif.

33. Swofford, D. L. 1993. PAUP (phylogenic analysis using parsimony). Laboratory of Molecular Systematics, National Museum of Natural History, Smithsonian Institution, Washington, D.C.

34. Versalovic, J., M. Schneider, F. J. deBruijn, and J. R. Lupski. 1994. Genomic fingerprinting of bacteria using repetitive sequence-based polymerase chain reaction. Methods Mol. Cell. Biol. 5:25-40.

35. Wells, J. M., B. C. Raju, H.-Y. Hung, W. G. Weisburg, L. Mandelco-Paul, and D. J. Brenner. 1987. Xylella fastidiosa gen. nov., sp. nov.: gram-negative, xylem-limited, fastidious plant bacteria related to Xanthomonas spp. Int. J. Syst. Bacteriol. 37:136-143[Abstract/Free Full Text].

36. Welsh, J., and M. McClelland. 1990. Fingerprinting genomes using PCR with arbitrary primers. Nucleic Acids Res. 18:7213-7218[Abstract/Free Full Text].

37. Wilson, K. 1987. Preparation of genomic DNA from bacteria, p. 2.4.1-2.4.2. In F. M. Ausubel, R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.), Current protocols in molecular biology. Greene Publishing Associates and Wiley Interscience, New York, N.Y.

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1.	Banks, D., R. Albibi, J. Chen, O. Lamikanra, R. L. Jarret, and B. J. Smith. 1999. Specific detection of Xylella fastidiosa Pierce's disease strains. Curr. Microbiol. 39:85-88[CrossRef][Medline].
2.	Barry, T., G. Colleran, M. Glennon, L. K. Dunican, and F. Gannon. 1991. The 16S/23S ribosomal spacer region as a target for DNA probes to identify eubacteria. PCR Methods Appl. 1:233-236.
3.	Chang, C. J., and N. W. Schaad. 1982. Electrophoretic protein profiles of total cell envelopes of xylem-limited plant pathogenic rickettsia-like bacteria (RLB). Phytopathology 72:935-936.
4.	Chen, J., C. J. Chang, and R. L. Jarret. 1992. Plasmids from Xylella fastidiosa. Can. J. Microbiol. 38:993-995.
5.	Chen, J., C. J. Chang, R. L. Jarret, and N. Gawel. 1992. Genetic variation among Xylella fastidiosa strains. Phytopathology 82:973-977.
6.	Chen, J., O. Lamikanra, C. J. Chang, and D. L. Hopkins. 1995. Randomly amplified polymorphic DNA analysis of Xylella fastidiosa Pierce's disease and oak leaf scorch pathotypes. Appl. Environ. Microbiol. 61:1688-1690[Abstract].
7.	Chu, G., D. Vollrath, and R. W. Davis. 1986. Separation of large DNA molecules by contour-clamped homogeneous electric fields. Science 234:1582-1585[Abstract/Free Full Text].
8.	Cooksey, D. A., and J. H. Graham. 1989. Genomic fingerprinting of two pathovars of phytopathogenic bacteria by rare-cutting restriction enzymes and field inversion gel electrophoresis. Phytopathology 79:745-750.
9.	da Costa, P. I., C. F. Franco, V. S. Miranda, D. C. Teixeira, and J. S. Hartung. 2000. Strains of Xylella fastidiosa rapidly distinguished by arbitrarily primed PCR. Curr. Microbiol. 40:279-282[CrossRef][Medline].
10.	Davis, M. J., W. J. French, and N. W. Schaad. 1981. Axenic culture of the bacteria associated with phony peach disease and plum leaf scald. Curr. Microbiol. 6:309-314[CrossRef].
11.	Davis, M. J., S. W. Thompson, and A. H. Purcell. 1979. Etiological role of the xylem-limited bacterium causing Pierce's disease in almond leaf scorch. Phytopathology 70:472-475.
12.	Felsenstein, J. 1993. PHYLIP (phylogeny inference package) version 3.5c. Department of Genetics, University of Washington, Seattle, Wash.
13.	Freitag, J. H. 1951. Host range of the Pierce's disease virus of grapes as determined by insect transmission. Phytopathology 41:920-934.
14.	Hewitt, W. B. 1958. The probable home of Pierce's disease virus. Plant Dis. Rep. 42:211-215.
15.	Hill, B. L., and A. H. Purcell. 1995. Acquisition and retention of Xylella fastidiosa by an efficient vector, Graphocephala atropunctata. Phytopathology 85:209-212.
16.	Hopkins, D. L. 1989. Xylella fastidiosa: xylem-limited bacterial pathogen of plants. Annu. Rev. Phytopathol. 27:271-290[CrossRef].
17.	Hopkins, D. L., and W. C. Adlerz. 1988. Natural hosts of Xylella fastidiosa in Florida. Plant Dis. 72:429-431.
18.	Jensen, M. A., J. A. Webster, and N. Straus. 1993. Rapid identification of bacteria on the basis of polymerase chain reaction-amplified ribosomal DNA spacer polymorphisms. Appl. Environ. Microbiol. 59:945-952[Abstract/Free Full Text].
19.	Kamper, S. M., W. J. French, and S. R. DeKloet. 1985. Genetic relationships of some fastidious xylem-limited bacteria. Int. J. Syst. Bacteriol. 35:185-188.
20.	Maniatis, T., E. F. Fritsch, and J. Sambrook. 1982. Molecular cloning $---$ a laboratory manual, p. 368-369. Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.
21.	Minsavage, G. V., C. M. Thompson, D. L. Hopkins, R. M. V. B. C. Leite, and R. E. Stall. 1994. Development of a polymerase chain reaction protocol for detection of Xylella fastidiosa in plant tissue. Phytopathology 84:456-461[CrossRef].
22.	Mircetich, S. M., S. L. Lowe, W. J. Moller, and G. Nyland. 1976. Etiology of almond leaf scorch disease and transmission of the casual agent. Phytopathology 66:17-24.
23.	Opgenorth, D. C., C. D. Smart, F. J. Louws, F. J. deBruijn, and B. C. Kirkpatrick. 1996. Identification of Xanthomonas fragariae field isolates by rep-PCR genomic fingerprinting. Plant Dis. 80:868-873.
24.	Pooler, M. R., and J. S. Hartung. 1997. Sequence analysis of a 1296-nucleotide plasmid from Xylella fastidiosa. FEMS Microbiol. Lett. 155:217-222[CrossRef][Medline].
25.	Pooler, M. R., J. S. Hartung, and R. G. Fenton. 1995. Genetic relationships among strains of Xylella fastidiosa from RAPD-PCR data. Curr. Microbiol. 31:134-137[CrossRef][Medline].
26.	Purcell, A. H. 1980. Almond leaf scorch: leafhopper and spittle bug vectors. J. Econ. Entomol. 73:834-838.
27.	Purcell, A. H. 1997. Xylella fastidiosa, a regional problem or global threat? J. Plant Pathol. 79:99-105.
28.	Purcell, A. H., S. R. Saunders, M. Hendson, M. E. Grebus, and M. J. Henry. 1999. Causal role of Xylella fastidiosa in oleander leaf scorch. Phytopathology 89:53-58[CrossRef].
29.	Rosato, Y. E., J. R. Neto, V. S. Miranda, E. F. Carlos, and G. P. Manfio. 1998. Diversity of a Xylella fastidiosa population isolated from Citrus sinensis affected by citrus variegated chlorosis in Brazil. Syst. Appl. Microbiol. 21:593-598.
30.	Sanger, F., S. Nicklen, and A. R. Coulson. 1977. DNA sequencing with chain termination inhibitors. Proc. Natl. Acad. Sci. USA 74:5463-5467[Abstract/Free Full Text].
31.	Simpson, A. A. J. G., F. C. Reinach, P. Arruda, F. A. Abreu, M. Acencio, R. Alvarenga, L. M. Alves, J. E. Araya, G. S. Baia, C. S. Baptista, et al. 2000. The genome sequence of the plant pathogen Xylella fastidiosa. Nature 406:151-157[CrossRef][Medline].
32.	Sneath, P. H. A., and R. R. Sokal. 1973. Numerical taxonomy. W. H. Freeman and Co., San Francisco, Calif.
33.	Swofford, D. L. 1993. PAUP (phylogenic analysis using parsimony). Laboratory of Molecular Systematics, National Museum of Natural History, Smithsonian Institution, Washington, D.C.
34.	Versalovic, J., M. Schneider, F. J. deBruijn, and J. R. Lupski. 1994. Genomic fingerprinting of bacteria using repetitive sequence-based polymerase chain reaction. Methods Mol. Cell. Biol. 5:25-40.
35.	Wells, J. M., B. C. Raju, H.-Y. Hung, W. G. Weisburg, L. Mandelco-Paul, and D. J. Brenner. 1987. Xylella fastidiosa gen. nov., sp. nov.: gram-negative, xylem-limited, fastidious plant bacteria related to Xanthomonas spp. Int. J. Syst. Bacteriol. 37:136-143[Abstract/Free Full Text].
36.	Welsh, J., and M. McClelland. 1990. Fingerprinting genomes using PCR with arbitrary primers. Nucleic Acids Res. 18:7213-7218[Abstract/Free Full Text].
37.	Wilson, K. 1987. Preparation of genomic DNA from bacteria, p. 2.4.1-2.4.2. In F. M. Ausubel, R. Brent, R. E. Kingston, D. D. Moore, J. G. Seidman, J. A. Smith, and K. Struhl (ed.), Current protocols in molecular biology. Greene Publishing Associates and Wiley Interscience, New York, N.Y.