Amplification of a 500-Base-Pair Fragment from Cultured Isolates of Mycobacterium bovis

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Journal of Clinical Microbiology, July 1999, p. 2330-2332, Vol. 37, No. 7
0095-1137/99/$04.00+0
Copyright © 1999, American Society for Microbiology. All rights reserved.

Amplification of a 500-Base-Pair Fragment from Cultured Isolates of Mycobacterium bovis

Juan Germán Rodríguez,¹^,^* Juan Carlos Fissanoti,² Patricia Del Portillo,¹ Manuel Elkin Patarroyo,³ María Isabel Romano,² and Angel Cataldi²

Corporación CorpoGen,¹ and Instituto de Inmunología, Hospital San Juan de Dios,³ Santafé de Bogotá, D.C. Colombia, and Instituto de Biotecnología CICV/INTA, Morón, Argentina²

Received 25 November 1998/Returned for modification 20 January 1999/Accepted 20 March 1999

	ABSTRACT

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The presence of a 500-bp fragment which amplifies a region from the genome of Mycobacterium bovis (J. G. Rodriguez, G. A.Meija, P. Del Portillo, M. E. Patarroyo, and L. A. Murillo, Microbiology141:2131-2138, 1995) was evaluated by carrying out PCR on 121M. bovis isolates. The M. bovis strains, previously characterizedby culture and biochemical tests, were isolated from cattle indifferent regions of Argentina, Mexico, and Colombia. Four additionalstrains isolated from sea lions that belong to the M. tuberculosiscomplex were also included in the study. All of the isolates testedwere PCR positive, rendering the expected 500-bp band and givinga correlation of 100% with previous microbiological characterization.Southern blot analysis revealed a common band of 1,800 bp anda polymorphic high-molecular-mass hybridization pattern. The resultsshow that this assay may be useful for diagnosis and identificationof M. bovis incattle.

	TEXT

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Bovine tuberculosis remains an important zoonosis in many countries of the world. Cases of human tuberculosis of bovine originhave increased in recent years (3, 5, 8, 19), and thiszoonosis has become a public health problem, as well as the causeof significant economic losses. Mycobacterium bovis, the causativeagent of bovine tuberculosis, infects both animals of agriculturalimportance and wild mammals, which act as a reservoir for theorganism, making it difficult to control the disease (12).

The bovine tuberculin test is easy to perform on a large scale on livestock, but it has the inconvenience of having a broadrange of specificity and sensitivity (13). Confirmation of thediagnosis is achieved by culture and biochemical assays. Despitethe fact that microbiological culture is highly specific, a positiveresult takes a long time to obtain and in most cases is achievedafter the animal has beensacrificed.

It is necessary to develop new diagnostic methods for bovine tuberculosis which could identify M. bovis directly in biologicalsamples, such as milk or blood, without having to culture themand which would also improve the predictive value of the tuberculintest. Although the PCR has been successfully applied for the diagnosisof tuberculosis, routine application of a PCR-based method requiresthat the target sequence be highly specific for the microorganismand that it be present in all of the strainsisolated.

Rodríguez et al. (14) reported a PCR assay which amplifies a 500-bp fragment from the M. bovis genome by using the JB21-JB22primer pair. However, only a small number of isolates were usedin that study. The present work was performed to determine whetherthis 500-bp fragment could be amplified from the genome of different,previously characterized, M. bovisisolates.

Mycobacterial isolates and DNA extraction. A total of 121 isolates identified as M. bovis on the basis of growth in the presence of pyruvate (scarce growth in glycerol),colony morphology, and biochemical and enzymatic tests (niacinnegative, nitrate reduction negative, catalase negative, ureasepositive, pyrazinamidase negative) were used in this study (9).Susceptibility to thiophene-2-carboxylic acid hydrazide and p-aminosalicylicacid was determined in egg solid medium with glutamate added andwithout glycerol (9). In some cases, guinea pigs and rabbitswere inoculated in order to confirm an M. bovis identification.M. tuberculosis H37Rv and M. bovis AN5 were used as referencestrains. One hundred twelve of these were bovine strains fromArgentina (taken from six different regions of the country), twowere bovine strains from Mexico, and seven were from Colombia.Four isolates belonging to the M. tuberculosis complex were obtainedfrom sea lions in Argentina and were also included in the study.Lymph nodes (40%), lung tissue (45%), liver (10%), and samplesfrom other locations (5%) were collected during necropsy and culturedin Stonebrink broth (16). All of them showed macroscopic lesionstypical of bovine tuberculosis. M. tuberculosis H37Rv, M. microti,M. africanum, and M. paratuberculosis were also analyzed in thestudy. Chromosomal DNAs were isolated as described by van Soolingenet al. (17), and 100 ng of each DNA was used for PCRamplification.

PCR assay. Primers JB21 and JB22 were synthesized on a Pharmacia synthesizer. Primer sequences and performance of the PCR were as reportedpreviously by Rodriguez et al. (14). The reactions were performedin a final volume of 50 µl containing 1× reaction buffer (Promega),2.5 U of Taq polymerase (Promega), 0.2 mM each deoxynucleosidetriphosphate, 1.5 mM magnesium chloride, and 20 pmol of each primer.Target DNA was denatured by incubation for 5 min at 94°C beforeamplification for 30 cycles of 94°C for 1 min, annealing at 68°Cfor 1 min, and extension at 72°C for 1 min. All reactions werecarried out in an automated thermal cycler (Biometra). After amplification,1/10 of the PCR mixture was analyzed by gel electrophoresis in1% agarose gels containing 0.5 µg of ethidium bromide perml.

Hybridization analysis. Genomic DNA was hydrolyzed with the PvuII restriction enzyme (Gibco BRL). After separation through agarose gel electrophoresis,the hydrolysate was transferred to a nylon membrane (Amersham)and hybridized with the 500-bp amplified fragment labeled with[ $alpha$ -³²P]dCTP by random priming (Rediprime;Amersham).

Results. PCR was carried out on 121 M. bovis isolates by using primers JB21 and JB22, which amplify a 500-bp fragment of M. bovis (14).The 500-bp genomic fragment was present in all of the M. bovisisolates used in this study, giving a 100% correlation with themicrobiological characterization. The fragment was also amplifiedfrom the genome of the four M. tuberculosis complex strains isolatedfrom sea lions. These isolates were characterized as M. tuberculosiscomplex strains because they shared molecular markers from bothM. tuberculosis and M. bovis (2, 15). No amplification wasobserved for M. tuberculosis H37Rv, M. africanum, M. microti,and four M. paratuberculosisstrains.

To determine whether this 500-bp sequence is present as a unique fragment in the M. bovis genome, Southern blot analysis wascarried out by using 17 M. bovis isolates selected as representativesof the total strains and the 500-bp fragment was used as a hybridizationprobe. As shown in Fig. 1, the 500-bp fragment hybridized to a1.8-kb band present in all of the samples tested, indicating acommon location within the M. bovis genome. In addition, positivesignals were obtained with one or two high-molecular-weight bands,between 7 and 10 kb. Hybridization with these high-molecular-weightbands was polymorphic among the different isolates tested andalso present when M. tuberculosis genomic DNA was used (data notshown).

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FIG. 1. Southern blot analysis of different isolates of M. bovis. Genomic DNA was digested with restriction enzyme PvuII, and the 500-bp fragment of M. bovis was used as a probe. Lanes 1 to 17 contain the following isolates of M. bovis: 1, 520; 2, 476; 3, 468; 4, 555; 5, 548; 6, 478; 7, T-372; 8, T-482; 9, 559; 10, 565; 11, 482; 12, 521; 13, 531; 14, 545; 15, 540; 16, 543; 17, 558. Lane 18 contains molecular weight markers. The values on the right are molecular weights in thousands.

Discussion. The accurate diagnosis of bovine tuberculosis remains, to this day, an elusive goal because no method has been developed whichcan precisely detect the presence of the microorganism in liveanimals. The tuberculin assay currently used around the worldrenders highly variable results due to problems with sensitivityand specificity. The tuberculin test depends on several factors,including high-quality reagents, as well as the immunologicalstatus of the animal. Furthermore, a negative tuberculin testdoes not means that the animal is not infected; on the other hand,a positive test can only mean a delayed hypersensitivity reactiondue to previous exposure. A PCR-based assay, such as the one describedhere, could be used to detect the presence of M. bovis in biologicalsamples (such as milk, blood, or nasal swabs) and thus becomean important tool for the control and eventual eradication ofthedisease.

A reliable PCR-based diagnostic assay must have a target DNA sequence that is specific for the microorganism to be detectedand that must also be present in most, if not all, isolates ofthe organism. The 500-bp fragment amplified by primers JB21 andJB22 fulfills the first requirement, since it is capable of discriminatingM. bovis from related strains, such as M. avium, which is commonlyisolated from cattle, and whose tuberculin is used in the comparativeintradermal tuberculin test, and M. paratuberculosis, which isalso pathogenic to cattle (1). This fragment also fulfillsthe second requirement: the results of this study confirm thatthe region amplified by primers JB21 and JB22 is conserved, sinceit was found in 121 isolates obtained from different geographicregions of Latin America. It is also important to note that theM. tuberculosis complex strains isolated from sea lions were PCRpositive, indicating that this sequence is also present in isolatesfrom other mammals, even thought they belong to a unique clusterclearly different from M. bovis strains, and closely related toM. tuberculosis (2, 4, 11, 15).

Initially, the fragment amplified by primers JB21 and JB22 was proposed by us to be exclusive to M. bovis and able to discriminatebetween M. bovis and M. tuberculosis. However, only 20 M. tuberculosisstrains were included in that study (14). As we included largernumbers of M. tuberculosis isolates, we have observed that thereare some strains which render a 500-bp amplification band withthe JB21-JB22 set of primers. This, however, does not necessarilydetract from the potential benefit of carrying out a PCR assaybased on this sequence in biological samples extracted from cattle,inasmuch as a positive amplification is indicative of the presenceof an infectious agent, be it human M. tuberculosis or M. bovisbovine tuberculosis. Studies are currently being carried out usinga large panel of M. tuberculosis strains to determine the percentageof JB21-JB22-positive amplifications. We are also using differentmolecular markers, such as spoligotyping (10), oxyR (7),and mtp40 (6), with the aim of determining whether these strainsmight belong to a cluster of M. tuberculosis, similar to whatis occurring with the sea lionisolates.

PCR-based assay has been successfully used for the detection of M. tuberculosis. Recently, however, it has been shown thatsome M. tuberculosis strains lack specific target sequences suchas IS6110 or mtp40 (11, 18). This could be due to the presenceof mutations or genomic rearrangements. So far, all of the M.bovis strains tested by the assay described here contain the 500-bptarget sequence, indicating that this fragment is conserved amongM. bovis strains. Field test evaluation of this PCR as a diagnostictool for M. bovis detection is being carried out by using milkand blood as biological samples in order to demonstrate the validityof the test for the detection of bovinetuberculosis.

	FOOTNOTES

^* Corresponding author. Mailing address: Corporación CorpoGen, Calle 26 A No. 37-28, Santafé de Bogotá, D.C. Colombia. Phone:57-1-368-5411. Fax: 57-1-3684987. E-mail: corpogen{at}colomsat.net.co.

REFERENCES

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Abstract
Text
References

1. Bauerfeind, R., S. Benazzi, R. Weiss, T. Schliesser, H. Willems, and G. Baljer. 1996. Molecular characterization of Mycobacterium paratuberculosis isolates from sheep, goats, and cattle by hybridization with a DNA probe to insertion element IS900. J. Clin. Microbiol. 34:1617-1621[Abstract].

2. Bernardelli, A., R. Bastida, P. Loureiro, C. Michelis, M. I. Romano, A. Cataldi, and E. Costa. 1996. Tuberculosis in sea lions and fur seals from the southwestern Atlantic Ocean. Rev. Sci. Tech. O. I. E. (Off. Int. Epizoot.) 15:985-1005.

3. Brett, J. L., and M. W. Humble. 1991. Incidence of human tuberculosis caused by Mycobacterium bovis. N. Z. Med. J. 104:13-14[Medline].

4. Cousins, D. V., B. R. Francis, B. L. Gow, D. M. Collins, C. H. McGlashan, A. Gregory, and R. M. Mackenzie. 1990. Tuberculosis in captive seals: bacteriological studies on an isolate belonging to the Mycobacterium tuberculosis complex. Res. Vet. Sci. 48:196-200[Medline].

5. de Kantor, I. N., and V. Ritacco. 1994. Bovine tuberculosis in Latin America and the Caribbean: current status, control and eradication programs. Vet. Microbiol. 40(1-2):5-14[Medline].

6. Del Portillo, P., L. A. Murillo, and M. E. Patarroyo. 1991. Amplification of a species-specific DNA fragment of Mycobacterium tuberculosis and its possible use in diagnosis. J. Clin. Microbiol. 29:2163-2168[Abstract/Free Full Text].

7. Espinosa de los Minteros, L. E., J. C. Galan, M. Gutierrez, S. Samper, J. F. Garcia Marin, C. Martin, L. Dominguez, L. de Rafael, F. Baquero, E. Gomez-Mampaso, and J. Blazquez. 1998. Allele-specific PCR method based on pncA and oxyR sequences for distinguishing Mycobacterium bovis from Mycobacterium tuberculosis: intraspecific M. bovis pncA sequence polymorphism. J. Clin. Microbiol. 36:239-242[Abstract/Free Full Text].

8. Fanning, A., and S. Edwards. 1991. Mycobacterium bovis infection in human beings in contact with elk (Cervus elaphus) in Alberta, Canada. Lancet 338:1253-1255[Medline].

9. Grange, J. M., and M. D. Yates. 1994. Guidelines for speciation within the Mycobacterium tuberculosis complex. WHO/Zoom./94.174. World Health Organization Veterinary Public Health Unit, Geneva, Switzerland.

10. Kamerbeek, J., L. Schouls, A. Kolk, M. van Agterveld, D. van Soolingen, S. Kuijper, A. Bunschoten, H. Molhuizen, R. Shaw, M. Goyal, and J. van Embden. 1997. Simultaneous detection and strain differentiation of Mycobacterium tuberculosis for diagnosis and epidemiology. J. Clin. Microbiol. 35:907-914[Abstract].

11. Liebana, E., A. Aranaz, B. Francis, and D. Cousins. 1996. Assessment of genetic markers for species differentiation within the Mycobacterium tuberculosis complex. J. Clin. Microbiol. 34:933-938[Abstract].

12. O'Reilly, L. M., and C. J. Daborn. 1995. The epidemiology of Mycobacterium bovis infection in animals and man: a review. Tubercle Lung Dis. 76:1-46.

13. O'Reilly, L. M. 1992. Specificity and sensitivity of tuberculin test, p. 83-139. In A. A. M. Moussa, O. Lotfi, S. Mahair, et al. (ed.), Proceedings of the International Conference on Animal Tuberculosis in Africa and the Middle East. General Organization for Veterinary Services, Cairo, Egypt.

14. Rodriguez, J. G., G. A. Mejia, P. Del Portillo, M. E. Patarroyo, and L. A. Murillo. 1995. Species-specific identification of Mycobacterium bovis by PCR. Microbiology 141:2131-2138[Abstract/Free Full Text].

15. Romano, M. I., A. Alito, F. Bigi, J. C. Fisanotti, and A. Cataldi. 1995. Genetic characterization of mycobacteria from South American wild seals. Vet. Microbiol. 47:89-98[Medline].

16. Stonebrink, B. 1958. The use of a pyruvate containing egg medium in the culture of isoniazid resistant strains of Mycobacterium tuberculosis var. Hominis. Acta Tuberc. Scand. 35:67-80.

17. Van Soolingen, D., P. W. M. Hermans, P. E. W. de Haas, D. R. Soll, and J. D. A. van Embden. 1991. The occurrence and stability of insertion sequences in Mycobacterium tuberculosis complex strains: evaluation of IS-dependent DNA polymorphism as a tool in the epidemiology of tuberculosis. J. Clin. Microbiol. 29:2578-2586[Abstract/Free Full Text].

18. Weil, A., B. B. Plikaytis, W. R. Butler, C. L. Woodley, and T. M. Shinnick. 1996. The mtp40 gene is not present in all strains of Mycobacterium tuberculosis. J. Clin. Microbiol. 34:2309-2311[Abstract].

19. World Health Organization. 1994. Zoonotic tuberculosis (Mycobacterium bovis): memorandum from a WHO meeting (with the participation of FAO). Bull. W. H. O. 72:851-857[Medline].

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1.	Bauerfeind, R., S. Benazzi, R. Weiss, T. Schliesser, H. Willems, and G. Baljer. 1996. Molecular characterization of Mycobacterium paratuberculosis isolates from sheep, goats, and cattle by hybridization with a DNA probe to insertion element IS900. J. Clin. Microbiol. 34:1617-1621[Abstract].
2.	Bernardelli, A., R. Bastida, P. Loureiro, C. Michelis, M. I. Romano, A. Cataldi, and E. Costa. 1996. Tuberculosis in sea lions and fur seals from the southwestern Atlantic Ocean. Rev. Sci. Tech. O. I. E. (Off. Int. Epizoot.) 15:985-1005.
3.	Brett, J. L., and M. W. Humble. 1991. Incidence of human tuberculosis caused by Mycobacterium bovis. N. Z. Med. J. 104:13-14[Medline].
4.	Cousins, D. V., B. R. Francis, B. L. Gow, D. M. Collins, C. H. McGlashan, A. Gregory, and R. M. Mackenzie. 1990. Tuberculosis in captive seals: bacteriological studies on an isolate belonging to the Mycobacterium tuberculosis complex. Res. Vet. Sci. 48:196-200[Medline].
5.	de Kantor, I. N., and V. Ritacco. 1994. Bovine tuberculosis in Latin America and the Caribbean: current status, control and eradication programs. Vet. Microbiol. 40(1-2):5-14[Medline].
6.	Del Portillo, P., L. A. Murillo, and M. E. Patarroyo. 1991. Amplification of a species-specific DNA fragment of Mycobacterium tuberculosis and its possible use in diagnosis. J. Clin. Microbiol. 29:2163-2168[Abstract/Free Full Text].
7.	Espinosa de los Minteros, L. E., J. C. Galan, M. Gutierrez, S. Samper, J. F. Garcia Marin, C. Martin, L. Dominguez, L. de Rafael, F. Baquero, E. Gomez-Mampaso, and J. Blazquez. 1998. Allele-specific PCR method based on pncA and oxyR sequences for distinguishing Mycobacterium bovis from Mycobacterium tuberculosis: intraspecific M. bovis pncA sequence polymorphism. J. Clin. Microbiol. 36:239-242[Abstract/Free Full Text].
8.	Fanning, A., and S. Edwards. 1991. Mycobacterium bovis infection in human beings in contact with elk (Cervus elaphus) in Alberta, Canada. Lancet 338:1253-1255[Medline].
9.	Grange, J. M., and M. D. Yates. 1994. Guidelines for speciation within the Mycobacterium tuberculosis complex. WHO/Zoom./94.174. World Health Organization Veterinary Public Health Unit, Geneva, Switzerland.
10.	Kamerbeek, J., L. Schouls, A. Kolk, M. van Agterveld, D. van Soolingen, S. Kuijper, A. Bunschoten, H. Molhuizen, R. Shaw, M. Goyal, and J. van Embden. 1997. Simultaneous detection and strain differentiation of Mycobacterium tuberculosis for diagnosis and epidemiology. J. Clin. Microbiol. 35:907-914[Abstract].
11.	Liebana, E., A. Aranaz, B. Francis, and D. Cousins. 1996. Assessment of genetic markers for species differentiation within the Mycobacterium tuberculosis complex. J. Clin. Microbiol. 34:933-938[Abstract].
12.	O'Reilly, L. M., and C. J. Daborn. 1995. The epidemiology of Mycobacterium bovis infection in animals and man: a review. Tubercle Lung Dis. 76:1-46.
13.	O'Reilly, L. M. 1992. Specificity and sensitivity of tuberculin test, p. 83-139. In A. A. M. Moussa, O. Lotfi, S. Mahair, et al. (ed.), Proceedings of the International Conference on Animal Tuberculosis in Africa and the Middle East. General Organization for Veterinary Services, Cairo, Egypt.
14.	Rodriguez, J. G., G. A. Mejia, P. Del Portillo, M. E. Patarroyo, and L. A. Murillo. 1995. Species-specific identification of Mycobacterium bovis by PCR. Microbiology 141:2131-2138[Abstract/Free Full Text].
15.	Romano, M. I., A. Alito, F. Bigi, J. C. Fisanotti, and A. Cataldi. 1995. Genetic characterization of mycobacteria from South American wild seals. Vet. Microbiol. 47:89-98[Medline].
16.	Stonebrink, B. 1958. The use of a pyruvate containing egg medium in the culture of isoniazid resistant strains of Mycobacterium tuberculosis var. Hominis. Acta Tuberc. Scand. 35:67-80.
17.	Van Soolingen, D., P. W. M. Hermans, P. E. W. de Haas, D. R. Soll, and J. D. A. van Embden. 1991. The occurrence and stability of insertion sequences in Mycobacterium tuberculosis complex strains: evaluation of IS-dependent DNA polymorphism as a tool in the epidemiology of tuberculosis. J. Clin. Microbiol. 29:2578-2586[Abstract/Free Full Text].
18.	Weil, A., B. B. Plikaytis, W. R. Butler, C. L. Woodley, and T. M. Shinnick. 1996. The mtp40 gene is not present in all strains of Mycobacterium tuberculosis. J. Clin. Microbiol. 34:2309-2311[Abstract].
19.	World Health Organization. 1994. Zoonotic tuberculosis (Mycobacterium bovis): memorandum from a WHO meeting (with the participation of FAO). Bull. W. H. O. 72:851-857[Medline].