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1 Sokoine University of Agriculture, Pest Management Centre, PO Box 3110, Morogoro, Tanzania
2 Royal Tropical Institute, Department of Biomedical Research, Meibergdreef 39, 1105 AZ Amsterdam, The Netherlands
Correspondence
G. F. Mgode
gfmgode{at}hotmail.com
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, 2003, 2004) showed that leptospirosis is much more common than generally thought. Currently, 20 Leptospira serovars from Africa have been described. Eleven of these serovars belong to the species Leptospira kirschneri, with eight being found in the Democratic Republic of Congo (Zaire), two in Kenya and one in Ghana (Faine et al., 1999). This suggests that L. kirschneri may be the prevalent Leptospira species, especially in Central and East Africa. Areas of high prevalence, such as Tanzania, might be harbouring many serovars which have not yet been described. Consistent with this assumption, we describe in this paper the isolation and identification of strain RM1 from cattle in Tanzania representing a new L. kirschneri serogroup Icterohaemorrhagiae proposed serovar, Sokoine.
Leptospira isolates and known pathogenic and saprophytic strains used in this study are listed in Table 1. Serovar Copenhageni, strain Wijnberg was used as reference pathogen, whereas serovars Semaranga and Patoc served as typical saprophytic reference strains. EMJH and Fletcher culture media were used to isolate and grow the leptospires (Faine, 1982). Leptospires were isolated from cattle in a slaughterhouse in Morogoro, Tanzania. Urinary bladders were aseptically punctured to obtain 0·5 ml aliquots of urine, which were then used to inoculate 5 ml Fletcher's medium, supplemented with 5-fluorouracil (200 µg ml–1) as a selective inhibitor of contaminating micro-organisms (Faine, 1982). Cultures were incubated at ambient temperatures (25–30 °C) and examined weekly over a period of 8 weeks using dark-field (DF) microscopy (Faine, 1982; Machang'u et al., 1997).
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and Johnson & Rogers (1964), respectively.
Briefly, 0·1 ml culture of isolate RM1 was used to inoculate 5 ml EMJH medium in four tubes and duplicates were incubated at 13 and 30 °C to determine the growth rates at low and high temperatures. EMJH medium (5 ml) with or without 8-azaguanine (225 µg ml–1) was inoculated in ‘duplicate’ with 0·1 ml isolate RM1 and then incubated at 30 °C to determine inhibition (reduction) of growth in the presence of 8-azaguanine. Leptospira growth was determined under DF microscopy and by measuring culture density at 420 nm spectrophotometrically (DU Series 62; Beckman Instruments). Pathogenic strain Wijnberg and saprophytic strain Patoc I (Table 1
) were included in the test for comparison of growth responses.
DNA was extracted from fully grown cultures using the Anansa Fast ‘n’ Easy Genomic DNA purification kit (Tebu-Bio Laboratories) and the method described by Boom et al. (1990). The quantity of extracted DNA was estimated by electrophoresis in a 1·5 % agarose gel stained with ethidium bromide by comparing the intensity of the genomic DNA bands with a standard DNA size marker (100–1000 bp, Smart ladder; Eurogentec). To determine the pathogenic status of the Leptospira isolate, PCR analysis was performed as described by Murgia et al. (1997) and Perolat et al. (1998). Primer pairs used included Lepat 1 and Lepat 2, which specifically amplify a 330 bp fragment from pathogenic leptospires, and Sapro 1 and Sapro 2, which specifically generate a 240 bp product from saprophytic leptospires (Murgia et al., 1997). Other primer pairs were LP1 and a1190 and LU and rLP, which amplify DNA from pathogenic leptospires producing specific amplicons of 1008 and 420 bp, respectively (Perolat et al., 1998).
PCR procedure described by Gravekamp et al. (1993) was used to determine whether isolate RM1 belonged to the species L. kirschneri. Primer pairs G1 and G2 that specifically amplify a 285 bp DNA fragment from all pathogenic Leptospira species, except L. kirschneri, and B64I and B64II that specifically amplify a 563 bp from L. kirschneri were used. Reference saprophytic and pathogenic strains were used as controls.
DNA fingerprinting was carried out as described previously (Zuerner et al., 1995; Zuerner & Bolin, 1997).
Primers derived from insertion element sequences IS1533 and IS1500, consisting of EPL-2 and EPR-2 and iP1 and iM16, respectively, were used separately and in combination. The generated DNA fingerprints of isolate RM1 and other Leptospira strains were compared following separation by electrophoresis in a 1·5 % agarose gel stained with ethidium bromide.
Isolate RM1 was subjected to serological microagglutination with 42 rabbit sera representative of all pathogenic and four saprophytic serogroups. The rabbit sera were prepared as described by Faine (1982) and the microagglutination test was carried out as described by Cole et al. (1973). Monoclonal antibody (mAb) typing was done using a panel of mAbs (F12C3-10, F20C3, F20C4-1, F52C1, F52C2, F70C4-1, F70C7-8, F70C13-1, F70C14-6, F70C20-3, F70C24-14, F70C26-1, F82C1-3, F82C2-2, F82C7-3, F82C8-4, F89C3-3 and F89C12-4) that characteristically agglutinate serovars belonging to serogroups Icterohaemorrhagiae and Sarmin as described by Korver et al. (1988). Reference serovars of Icterohaemorrhagiae and Sarmin groups (Table 1) were included in this test for comparison of their agglutination patterns with that of isolate RM1.
Cross-agglutination absorption test (CAAT), the gold standard test for serological classification of Leptospira serovars, was repeatedly carried out by the Sokoine University of Agriculture (Tanzania) as described elsewhere (Stallman, 1987; Dikken & Kmety, 1978). CAAT results were confirmed by the WHO/FAO/OIE Collaborating Centre for Reference and Research on Leptospirosis of the Royal Tropical Institute, Amsterdam, The Netherlands.
Results from this study revealed that isolate RM1 is a pathogenic Leptospira as indicated by suppressed growth both at 13 °C and in the presence of 8-azaguanine. PCR with pathogenic primers Lepat 1 and Lepat 2 gave a DNA product of 330 bp (Supplementary Fig. S1 available in IJSEM Online). No DNA product was generated using the saprophytic Leptospira-specific primers Sapro 1 and Sapro 2 (data not shown). In addition, a 1008 bp PCR product was obtained with the primers LP1 and a1190 (Supplementary Fig. S2 available in IJSEM Online) and a 420 bp DNA product was obtained with primer pair LU and rLP (data not shown). These findings support the pathogenic status of RM1. Strain RM1 was PCR-positive with an L. kirschneri-specific primer pair (B64I and B64II) by generating an amplicon of 563 bp, while no product was generated with primers G1 and G2 (data not shown). This suggests that RM1 is a strain of the species L. kirschneri (Gravekamp et al., 1993). PCR-based fingerprinting with primer iM16 derived from IS1500 produced a pattern from RM1 DNA which was closely related to that of serovar Ndahambukuje and somewhat related to L. kirschneri and Leptospira interrogans strains (data not shown). Distinct DNA patterns were obtained from serovar Ndambari and Bogvere that produced few bands for comparison. Apparently, RM1 is genotypically closely related to serovar Ndahambukuje. However, the iM16-based fingerprinting was not informative enough to explain the genetic relatedness of these serovars. DNA fingerprinting with primers derived from IS1533 (EPL-2 and EPR-2) did not yield DNA profiles with multiple bands from L. kirschneri strains included in the analysis to enable comparison (data not shown). This probably suggests that there are only a few copies of the IS1533 element in these strains.
Sero-agglutination was observed with sera specific for serogroups Icterohaemorrhagiae, Canicola and Sarmin. Further agglutination tests with rabbit sera against individual serovars of each of the three groups revealed highest agglutination titres with 13 of 17 serovars of the Icterohaemorrhagiae group, one of six serovars of the Sarmin group and one of 13 serovars of the Canicola group. These findings suggest that RM1 most likely belongs to the serogroup Icterohaemorrhagiae or to the serologically closely related serogroup Sarmin.
Subsequent typing with a panel of mAbs, which characteristically agglutinate serovars of the serogroups Icterohaemorrhagiae and Sarmin, revealed the highest similarity with serovars from the Icterohaemorrhagiae group, while the relationship with the Sarmin group was virtually ruled out (data not shown). Therefore, we conclude that RM1 represents a serovar of serogroup Icterohaemorrhagiae. The agglutination profile obtained with RM1 was not identical to that of any of the established serovars of serogroup Icterohaemorrhagiae. Best fits were found with the histograms of serovars Ndahambukuje and Ndambari (Supplementary Figs S3 and S4 available in IJSEM Online). These observations suggest RM1 to be a new serovar of the Icterohaemorrhagiae group.
CAAT was performed repeatedly with serovars of serogroup Icterohaemorrhagiae, of which the rabbit sera showed high cross-agglutination titres (>10 % compared with the homologous titre) with RM1 and vice versa. CAAT results (Table 2) indicate that none of the rabbit sera, after heterologous absorption, give a remaining titre of less than 10 % in both forward and reverse reactions. According to the definition of the subcommittee on the taxonomy of Leptospira (Stallman, 1987), this finding further shows that RM1 represents a new serovar of serogroup Icterohaemorrhagiae.
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). Additionally, serovar Sokoine is genotypically closely related to serovar Ndahambukuje, although the IS1500 and IS1533 fingerprints did not provide enough DNA profiles to conclude on the level of relationships. It might be hypothesized that the observed serological and genotypic relationship between the L. kirschneri serovars Ndahambukuje and Ndambari and the proposed serovar Sokoine from Tanzania suggests that these serovars evolved from a common ancestor, composing a prevalent group of related serovars in East and Central Africa and possibly have cattle as a natural host. Further studies will be needed to confirm this hypothesis. These findings agree with the prevalence of L. kirschneri in Africa (Faine et al., 1999).
Short description of Leptospira serovar Sokoine
The proposed Leptospira serovar Sokoine strain RM1 was isolated from cattle in a slaughterhouse in Morogoro, Tanzania. Serovar Sokoine is deposited under its own serovar and strain name (no accession number) in two Leptospira culture collection centres: (i) the WHO/FAO/OIE Collaborating Centre for Reference and Research on Leptospirosis of the Royal Tropical Institute, Amsterdam, The Netherlands, and (ii) the WHO Collaboration Centre for Diagnosis, Reference, Research and Training in Leptospirosis, Port Blair, Andaman and Nicobar Islands, India. RM1 grows well in Leptospira culture media (Fletcher's and EMJH) at ambient temperatures. Growth of this strain is inhibited at 13 °C and by 8-azaguanine, which is consistent with pathogenic status. Genomic DNA of strain RM1 is PCR-positive with primers designed for pathogenic leptospires and with specific primers for amplifying DNA from strains of L. kirschneri. Serovar Sokoine is distinct from all other recognized serovars of the Icterohaemorrhagiae group on the basis of the CAAT results. It gives highest titres in agglutination with antibodies to various serovars of the Icterohaemorrhagiae group, and hence can serve as broad antigen for preliminary serological diagnosis of infection with leptospires of the Icterohaemorrhagiae group.
This isolate can be classified as L. kirschneri serogroup Icterohaemorrhagiae serovar Sokoine strain RM1. The naming of serovar Sokoine is given in the honour of the Sokoine University of Agriculture in Morogoro, Tanzania, where research on leptospirosis in Tanzania was pioneered.
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ACKNOWLEDGEMENTS |
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REFERENCES |
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Brenner, D. J., Kaufmann, A. F., Sulzer, K. R., Steigerwalt, A. G., Rogers, F. C. & Weyant, R. S. (1999). Further determination of DNA relatedness between serogroups and serovars in the family Leptospiraceae with a proposal for Leptospira alexanderi sp. nov. and four new Leptospira genomospecies. Int J Syst Bacteriol 49, 839–858.
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