Genetic Classification of "Rickettsia heilongjiangii" and "Rickettsia hulinii," Two Chinese Spotted Fever Group Rickettsiae

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Journal of Clinical Microbiology, September 2000, p. 3498-3501, Vol. 38, No. 9
0095-1137/00/$04.00+0
Copyright © 2000, American Society for Microbiology. All rights reserved.

Genetic Classification of "Rickettsia heilongjiangii" and "Rickettsia hulinii," Two Chinese Spotted Fever Group Rickettsiae

J. Z. Zhang,¹^,² M. Y. Fan,² Y. M. Wu,³ P. E. Fournier,¹ V. Roux,¹ and D. Raoult¹^,^*

Unité des Rickettsies, Faculté de Médecine, CNRS UPRES-A6020, 13385 Marseille Cedex 05, France,¹ and Department of Rickettsiology, Institute of Epidemiology & Microbiology, Chinese Academy of Preventive Medicine, Beijing 102206,² and Department of Microbiology, Institute of Military Medicine, Shengyang Military Command, Shengyang 110034,³ Peoples Republic of China

Received 24 January 2000/Returned for modification 2 May 2000/Accepted 5 July 2000

	ABSTRACT

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To determine the phylogenetic position of two new rickettsial strains isolated from ticks in China, 16S ribosomal DNA, gltA,and ompA (apart from the tandem repeat units) genes were amplifiedby PCR and sequenced. The phylogenetic relationships between thesestrains and other rickettsiae were inferred from the comparisonof sequences of the three genes by the parsimony, neighbor-joining,and maximum-likelihood methods. The results demonstrated thatthe 054 strain, a rickettsia pathogenic in humans, and the HL-93strain were related and clustered together with Rickettsia japonica.Significant statistical bootstrap values (100 and 92%) supportedthe nodes in this cluster. Based on previous genotypic and antigenicdata and the phylogenetic analysis presented here, the 054 andHL-93 strains should be considered as new species, and we formallypropose that they be named "Rickettsia heilongjiangii" and "Rickettsiahulinii,"respectively.

	TEXT

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The advent of new culture techniques, such as the shell vial-centrifugation technique (16), and the detection of rickettsialDNA have dramatically increased the number of rickettsial speciesdetected (20). Before 1984, only six spotted fever group (SFG)rickettsioses were recognized in the world (20): Rocky Mountainspotted fever caused by Rickettsia rickettsii, Mediterranean spottedfever caused by Rickettsia conorii, Siberian tick typhus causedby Rickettsia sibirica, Queensland tick typhus caused by Rickettsiaaustralis, rickettsialpox caused by Rickettsia akari, and Israelispotted fever caused by Israeli tick typhus rickettsia. Over thelast 12 years, eight new rickettsioses have been reported, includingJapanese spotted fever caused by Rickettsia japonica, FlindersIsland spotted fever caused by Rickettsia honei, Astrakhan fevercaused by Astrakhan fever rickettsia, African tick bite fevercaused by Rickettsia africae, California flea typhus caused bythe ELB agent, and three unnamed spotted fevers caused by "Rickettsiamongolotimonae," Rickettsia slovaca, and Rickettsia helvetica.In China, 20 strains of tick-associated rickettsiae, belongingto at least five serotypes, have been isolated over the last fewyears, including R. sibirica; the BJ-90 isolate (42); the Heilongjiangisolate (strain 054, also called "Rickettsia heilongjiangii");the Inner Mongolian isolate HA-91, or "R. mongolotimonae," alsofound in France; and the Hulin isolate (strain HL-93, also called"Rickettsia hulinii") (9, 19, 33). Three of these rickettsiae,R. sibirica, "R. mongolotimonae," and "R. heilongjiangii," arehuman pathogens. "R. heilongjiangii" was first isolated in 1982from Dermacentor silvarum ticks collected in Suifenhe, a cityof Heilongjiang Province in China (Fig. 1). Between May and July1988, 12 patients in Chunhua, Huichun County, Jilin Province,were reported to be infected by this strain on the basis of serologicalresults. All patients had a history of fever, headache, rash,eschar, regional lymphadenopathy, and conjunctivitis followinga tick bite, with fourfold rises in complement fixation antibodiesin convalescent-phase sera (14). Between May and June 1996,seven patients with clinical manifestations of SFG rickettsialinfections were found in Suifenhe and Dongning, in HeilongjiangProvince. Isolates from these patients were found to be identicalto the 054 strain by microimmunofluorescence and PCR plus restrictionfragment length polymorphism (30). The "R. hulinii" strain wasfirst isolated in 1993 from Haemaphysalis concinna ticks collectedin Hulin County, Heilongjiang Province (Fig. 1), and was consideredto be a unique SFG rickettsia (38). To date, the pathogenicityof this strain has been experimentally demonstrated in animals(38), but not in humans. In order to estimate the phylogeneticclassification of strains 054 and HL-93, we sequenced their 16SrRNA (16S ribosomal DNA [rDNA])-, citrate synthase (gltA)-, andrOmpA (ompA)-encoding genes and compared these sequences withthose of other SFG rickettsiae.

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FIG. 1. Map of China showing the areas of collection of ticks from which strains 054 and HL-93 were isolated.

Strains 054 and HL-93 were cultivated and purified as previously described (12), and their DNA was extracted from purifiedorganisms with the QIAmp tissue kit (Qiagen, Hilden, Germany)according to the manufacturer's instructions. PCR amplificationand sequencing reactions were performed with the oligonucleotideprimers mentioned below. All primers were purchased from GIBCOBRL (Custom Primers, Life Technologies Sarl. B.P., Cergy PontoiseCedex, France), and amplifications were carried out in a Peltiermodel PTC-200 DNA thermal cycler (MJ Research, Inc., San Francisco,Calif.) under conditions previously described (11, 22-24). R.japonica and distilled water were used as a positive and negativecontrol, respectively. Each amplicon obtained was purified forsequencing with a QIAquick Spin PCR Purification kit (Qiagen,Courtaboeuf, France) according to the manufacturer's protocol.Sequencing reactions were carried out with the Dye Terminatorkit (D-rhodamine terminator cycle DNA sequencing kit; Perkin-Elmer)as described by the manufacturer. Sequencing reaction productswere resolved by electrophoresis with an ABI Prism 377 Sequencer(Perkin-Elmer). The results obtained were processed into sequencedata by using the Sequence Navigator and AutoAssembler software.Each base position was established at least three times in boththe forward and reverse directions. Sequences of the 16S rDNA,gltA, and ompA genes were aligned by using the multisequence alignmentprogram CLUSTAL, within the BISANCE environment (7). Phylogeneticrelationships between strains 054 and HL-93 and other SFG rickettsiaewere inferred by using version 3.4 of the PHYLIP software package(10). The distance matrices generated by DNADIST were determinedunder the assumptions of Kimura (13) and were used to inferdendrograms by the neighbor-joining method (25). Two other dendrogramswere constructed by data processing with the maximum-likelihoodand parsimony programs in PHYLIP. A bootstrap analysis based on100 randomly generated trees by using SEQBOOT and CONSENSE inPHYLIP was performed to estimate the node reliability of the treesobtained by the three phylogenetic methods (4).

The primers fD1 and rP2 amplified 1,463- and 1,461-bp fragments of the 16S rDNA gene from strains 054 and HL-93, respectively.The gltA gene was amplified in two fragments. Overall, sequencesof 1,238 and 1,237 bp were obtained from the O54 and HL-93 strains,respectively. PCR amplification and sequencing of the ompA geneexcluded the central tandemly repeat region. The 5'-end fragmentof the gene was 611 bp for both the 054 and HL-93 strains. The3' part of the gene was amplified in four fragments. Overall,sequences of 3,187 and 3,181 bp were obtained from strains 054and HL-93, respectively. The sequenced fragments of the rOmpAgene were analyzed from base positions 91 to 680 and 3608 to 6789with respect to the sequence published for R. rickettsii (2)and were therefore submitted to GenBank as two separate fragments.Strains 054 and HL-93 clustered together with R. japonica intoa well-defined, strongly supported monophyletic group within theSFG rickettsiae, with bootstrap values of 91 and 100% for thenode where strains and HL-93 branched together in the gltA andompA trees, respectively, and values of 92 and 100% for the nodewhere both strains clustered with R. japonica. Similar phylogeneticorganizations were inferred from the analysis of all three genesby using the three phylogenetic analysis methods (Fig. 2).

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FIG. 2. Dendrogram representing phylogenetic relationships between Rickettsia species inferred from the comparison of gltA (left) and ompA (right) sequences by the neighbor-joining method. The bootstrap values are indicated at the nodes.

Historically, the classification and identification of rickettsiae have been based on differences in their epidemiology, serology,and intracellular growth characteristics. Because different speciesmay have common ecological features (e.g., geographic distribution,arthropod vectors, etc.) and due to serological cross-reactivity,it is difficult to distinguish between rickettsiae. Moreover,DNA-DNA hybridization, a criterion used for the definition ofspecies in the family Enterobacteriaceae, is not applicable toSFG rickettsiae (8). Other recognized tools for the taxonomicclassification of bacteria, such as the study of protein profilesby sodium dodecyl sulfate-polyacrylamide gel electrophoresis,monoclonal antibodies, Western blotting, and hybridization oflabeled cloned DNA probes (1, 3, 17, 21, 31, 32,34), are not widely applicable and lack interlaboratory reproducibility.Therefore, for over 10 years, the reference method for the identificationof members of SFG rickettsiae has been the indirect microimmunofluorescenceserologic typing test with mouse sera (18). Recently, phylogeneticanalyses and the determination of taxonomic relationships basedon comparisons of sequences of a combination of various geneshave greatly facilitated the study of rickettsial taxonomy. The16S rDNA (23, 26, 28), gltA (24), and ompA (11, 22)genes appear to be the most useful sequences. In our study, the054 and HL-93 strains demonstrated ompA sequence homologies of98.1% with each other and 96.6 and 95.6% with R. japonica, respectively,which are higher than those observed for strain HL-93 with R.rickettsii or R. conorii (94 and 90%, respectively). Althoughclosely related, the data from our study show that strains 054and HL-93 are distinct species (Fig. 2). Strains 054 and HL-93and R. japonica were grouped into a well-supported cluster inthe phylogenetic trees developed by the three analysis methods(Fig. 2). These results are the first showing isolates clusteringwith R. japonica and are in concordance with previous phenotypicand genotypic studies (5, 6, 15, 29, 30, 35-41; L.Chen, J. Z. Zhang, and D. Z. Bi, Program Abstr. EUWOG-ASR JointMeeting, p. 12, 1999). Tick-associated rickettsiae are characterizedby limited, specific geographical distribution areas (11). R.japonica was first isolated on Shikoku Island (27), the smallestof Japan's four main islands. The island is located between 132°to 135° East and 33° to 35° North. To the north is the Seto InlandSea, while to the south is the Pacific Ocean. Heilongjiang Provinceof China, where the 054 and HL-93 strains were isolated, is locatedbetween about 130° to 140° East and 45° to 50° North. This suggeststhat an SFG rickettsia may have evolved separately in this areaof the world and diverged more recently into Japan and in China.The current rickettsial taxonomy is based on serotyping (11),and, to date, there is no consensus on alternative genomic tools.However, based on data from previous genotypic and antigenic studiesand on the phylogenetic analysis presented here, we believe thatthe 054 and HL-93 strains should be strongly considered as membersof new species, and we formally propose that these be named "Rickettsiaheilongjiangii" and "Rickettsia hulinii,"respectively.

Nucleotide sequence accession numbers. The 16S rDNA GenBank accession numbers are AF172942 and AF178037 for 054 and HL-93, respectively. The gltA accessionnumbers are AF178034 and AF172943 for 054 and HL-93, respectively.The ompA accession numbers are AF179362 and AF179364 forthe 5' fragments of 054 and HL-93, respectively, and AF179363and AF179366 for the 5' fragments of 054 and HL-93,respectively).

	FOOTNOTES

^* Corresponding author. Mailing address: Unité des Rickettsies, Faculté de Médecine, CNRS UPRES-A6020, 13385 Marseille Cedex05, France. Phone: (33) 491 32 43 75. Fax: (33) 491 83 03 90.E-mail: Didier.Raoult{at}medecine.univ-mrs.fr.

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1.	Anacker, R. L., R. N. Philip, J. C. Williams, R. H. List, and R. E. Mann. 1984. Biochemical and immunochemical analysis of Rickettsia rickettsii strains of various degrees of virulence. Infect. Immun. 44:559-564[Abstract/Free Full Text].
2.	Anderson, B. E., G. A. MacDonald, D. C. Jones, and R. L. Regnery. 1990. A protective protein antigen of Rickettsia rickettsii has tandemly repeated, near-identical sequences. Infect. Immun. 58:2760-2769[Abstract/Free Full Text].
3.	Anderson, B. E., and T. Tzianabos. 1989. Comparative sequence analysis of a genus-common rickettsial antigen gene. J. Bacteriol. 171:5199-5201[Abstract/Free Full Text].
4.	Brown, J. K. M. 1994. Bootstrap hypothesis tests for evolutionary trees and other dendrograms. Proc. Natl. Acad. Sci. USA 91:12293-12297[Abstract/Free Full Text].
5.	Chen, M., M. Y. Fan, D. Z. Bi, and J. Z. Zhang. 1998. Sequence analysis of a fragment of rOmpA gene of several isolates of spotted fever group rickettsiae from China. Acta Virol. 42:91-93[Medline].
6.	Chen, X. R., Z. P. Xu, W. R. Chen, S. L. Li, and Y. G. Zhang. 1997. Studies on the features of the strains of spotted fever group rickettsiae. Microbiology 24:31-31.
7.	Dessen, P., C. Fondrat, C. Valencien, and G. Munier. 1990. BISANCE: a French service for access to biomolecular databases. CABIOS 6:355-356[Free Full Text].
8.	Drancourt, M., and D. Raoult. 1994. Taxonomic position of the rickettsiae: current knowledge. FEMS Microbiol. Rev. 13:13-24[CrossRef][Medline].
9.	Fan, M. Y., J. Z. Zhang, M. Chen, and X. J. Yu. 1999. Spotted fever group rickettsioses in China, p. 247-257. In D. Raoult, and P. Brouqui (ed.), Rickettsiae and rickettsial diseases at the turn of the third millenium. Elsevier, Paris, France.
10.	Felsenstein, J. 1989. PHYLIP $---$ phylogeny inference package (version 3.2). Cladistics 5:164-166.
11.	Fournier, P. E., V. Roux, and D. Raoult. 1998. Phylogenetic analysis of spotted fever group rickettsiae by study of the outer surface protein rOmpA. Int. J. Syst. Bacteriol. 48:839-849[Abstract/Free Full Text].
12.	Hanson, B. A., C. L. Wisseman, Jr., A. Waddell, and D. J. Silverman. 1981. Some characteristics of heavy and light bands of Rickettsia prowazekii on Renografin gradients. Infect. Immun. 34:596-604[Abstract/Free Full Text].
13.	Kimura, M. 1980. A simple method for estimating evolutionary rate of base substitutions through comparative studies of nucleotide sequences. J. Mol. Evol. 16:111-120[CrossRef][Medline].
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