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Heterogeneidade de resposta por IFN-γ a cepas clínicas de Mycobacterium tuberculosis em humanos

Heterogeneidade de resposta por IFN-γ a cepas clínicas de Mycobacterium tuberculosis em humanos

Vinícius Ribeiro Cabral, Cláudia Ferreira de Souza, Fernanda Luiza Pedrosa Guimarães, Maria Helena Feres Saad

ABSTRACT

Mycobacterium tuberculosis is one of the most successful human pathogens. Highly virulent strains, which are more easily transmitted than are less virulent strains, elicit variable immune responses. We evaluated the Th1 responses (IFN-γ production) in healthy volunteers after stimulation with various strains. Our results show that the individuals with negative tuberculin skin test (TST) results were not necessarily naive to all of the strains tested, whereas individuals with positive TST results did not respond to all of the strains tested. Drug-resistant strains induced a lower mean level of IFN-γ production than did drug-sensitive strains. One possible practical application of this finding would be for the prediction of responses to treatment, in which it might be advantageous to have knowledge of the estimated IFN-γ production elicited by a specific isolated strain.

Keywords: Tuberculosis; Polymorphism, restriction fragment length; Mycobacterium tuberculosis; Immunity, cellular; Interferon-gamma.

RESUMO

Mycobacterium tuberculosis é um dos mais bem sucedidos patógenos do homem. As cepas virulentas são mais facilmente transmitidas, induzindo respostas imunes variáveis. Avaliamos a resposta celular tipo Th1, através da produção de IFN-γ, como resposta a cepas com padrões diversos em voluntários sadios. Nossos resultados mostraram que indivíduos com teste tuberculínico (TT) negativo já tiveram contato com algumas das cepas testadas, ao passo que indivíduos com TT positivo não responderam a todas as cepas testadas. Cepas resistentes induziram uma média menor de produção de IFN-γ que aquelas sensíveis. Uma possível aplicação prática disto seria que a produção de IFN-γ, em relação a uma cepa isolada específica, poderia auxiliar na previsão da resposta ao tratamento dos pacientes.

Palavras-chave: Tuberculose; Polimorfismo de fragmento de restrição; Mycobacterium tuberculosis; Imunidade celular; Interferon gama.

According to the World Health Organiza­tion,(1) based on a hypersensitivity response to PPD, approximately one third of the world population is infected with Mycobacterium tuberculosis. Paradoxically, the human immune response is quite efficient in defeating the growth of this pathogen but is not efficacious in its eradication. The natural history of tuberculosis indicates that only 10% of infected individuals are at risk of developing the disease at some point in their life. However, the majority of infected individuals might be in jeopardy of reactivation of the disease when the immune system becomes suppressed or when there is reinfection with a new strain. Some studies have demonstrated a correlation between M. tuberculosis virulence and lack of Th1 response in murine models. Others have suggested that certain strains, typically those with special features, such as the Beijing strain, interact distinctly with the host, inducing different immune responses according to their transmission potential.(2,3) In the present study, we assessed the ability of clinical and nonclinical isolates of drug-resistant or drug-sensitive M. tuberculosis strains to induce IFN-γ-mediated protective immune responses in healthy volunteers. The study design was approved by the institutional research ethics committee.

The clinical strains were isolated from patients with pulmonary tuberculosis. The H37Rv strain of M. tuberculosis was obtained from the American Type Culture Collection (Manassas, VA, USA). The characteristics of the various strains are described in Table 1. The susceptibility test was performed by the Löwenstein-Jensen (LJ) proportion method,(4) and the insertion sequence 6110 (IS6110) pattern was obtained by RFLP.(5,6) We recruited 11 healthy volunteers, all of whom underwent a tuberculin skin test (TST). Of those 11 volunteers, 6 tested positive (TST+, induration ≥ 5 mm) and 5 tested negative (TST−). None of the volunteers had a history of tuberculosis. All of the volunteers gave written informed consent.




Blood samples were drawn, and PBMCs were prepared as described by Tavares et al.(7) In-vitro stimulation of 106 cells/well was accomplished via incubation, for three days, with a suspension containing 105 bacilli/well, and, as a positive control, 5 µg/mL of PHA (Sigma, St. Louis, MO, USA). Supernatants of bacteria-free cell cultures were collected and stored immediately at −70°C for IFN-γ quantification using ELISA (R&D Systems, Minneapolis, MN, USA). Levels of IFN-γ > 100 pg/mL were considered positive. The suspension of bacilli was prepared by cultivating the strains for three weeks at 37°C on LJ medium. The fresh growth was removed, placed into a tube containing 3-mm glass beads, and vortexed for 1 min. Following the addition of 5% PBS-Tween 80, mycobacterial growth was dispersed (by multiple aspirations with a 25-gauge needle), vortexed, and twice washed thoroughly in PBS by centrifugation. Remaining large particles were allowed to settle for 30 min, after which the supernatant cell count was adjusted to a McFarland standard of 1 and then to the desired number. Clump-free cell suspension was verified by smear microscopy for AFB. Results are expressed as mean ± SE. Data were analyzed by the nonparametric Student's t-test. The cut-off point for IFN-γ was 100 pg/mL, unless the background levels were higher in the unstimulated control cells, in which case a value at least twice that of the control was considered positive.

Table 2 shows the IFN-γ production after stimulation with the various strains. As expected, most of the TST+ volunteers produced IFN-γ in response to stimulation with the strains tested. Despite the fact that some of the strains tested have yet to be recognized, the intensity of the response, in most cases, correlated positively with the size of the induration on the TST. The multidrug-resistant M. tuberculosis strain 046, harboring ten IS6110 copies and belonging to a cluster, was the strain most often evoking an immune response in the sample as a whole and even evoked such a response in 1 (20%) of the 5 TST− volunteers. This indicates that some of the healthy individuals, despite being TST−, were not naive to all M. tuberculosis strains, although it might indicate a cross-reaction with environmental mycobacteria. It is known that PPD and H37Rv antigens induce Th1 responses in TST+ individuals. One TST− volunteer had a cytokine response to the H37Rv strain and to one other strain. However, in the sample as a whole, elevated IFN-γ production correlated with the TST induration, except in the case of one TST+ individual (volunteer I), in whom neither H37Rv nor any of the other strains elicited IFN-γ production. The fact that some TST+ individuals from endemic areas did not respond to mycobacterial strains might be relevant in vaccine testing, as well as in the use of diagnostic methods based on the IFN-γ response assay, which have been commercially used to identify individuals with latent tuberculosis infection. Because certain clinical isolates, including H37Rv, produce a variety of responses in humans, as well as because virtually all new tuberculosis vaccines (most of which contain the H37Rv strain) are tested in animals, it remains unknown whether new vaccines (targeting other strains) will provide the same level of protection as that observed for those targeting this standard strain. Recently, clinical M. tuberculosis strains have been reported to produce a variable disease response in animal models.(8) Further studies are needed in order to elucidate the influence that the estimated sensitivity of the IFN-γ response assay has on INF-γ levels in individuals with latent tuberculosis infection.




The isoniazid-resistant strain 238, harboring a cluster with two copies of IS6110, induced IFN-γ production in only 2 of the volunteers (volunteers G and K), who presented with low positivity for IFN-γ and TST indurations of 10 and 20 mm, respectively. Among the TST+ volunteers, the mean level of IFN-γ production was lower for the drug-resistant strains than for the drug-susceptible strains (445.6 ± 155.6 pg/mL vs. 548.10 ± 153.9 pg/mL). The same was observed among the TST− volunteers (43.78 ± 12.73 pg/mL vs. 51.72 ± 14.25 pg/mL), although the difference was not significant. According to previous reports, some prevalent endemic strains, as well as those with low IS6110 copy numbers, might have higher virulence and greater transmission potential, being associated with a lack of a protective immune response, as well as with the suppression of IL-1β, IFN-γ, and TNF-α production.(9-11) In the present study, clustered strains less often evoked an immune response from TST+ volunteers. However, all of the clustered strains isolated were drug-resistant strains. Decreased IFN-γ production has previously been described in patients infected with multidrug-resistant strains.(12,13) Our study produced similar results, which corroborates reports that drug-resistant strains downregulate the Th1 response, and that the degree of downregulation is strain-dependent.

In summary, we observed heterogeneous cytokine immune responses for a panel of clinical M. tuberculosis strains. This suggests a strain-to-strain difference in virulence factors. In general, an effective immune response is more likely to depend on the host than on the infecting strain. However, we observed some particular responses related to strain characteristics such as drug resistance. This suggests that an estimate of the IFN-γ production elicited by a specific isolated strain might help predict the response to treatment. In our study, some strains were shown to induce or mimic severe disease by downregulating the IFN-γ response, which can have implications for the efficacy of T cell-based diagnostic tests. In addition, our results suggest that new vaccines should be evaluated as to whether they elicit immune responses to other M. tuberculosis strains, since we have demonstrated that the characteristic clinical strains evoke heterogeneous host responses.

Acknowledgments

We thank Mitchell Raymond Lisbon for reviewing the English grammar.


References


1. World Health Organization. Global tuberculosis control: surveillance, planning, financing. Geneva: World Health Organization; 2007.

2. López B, Aguilar D, Orozco H, Burger M, Espitia C, Ritacco V, et al. A marked difference in pathogenesis and immune response induced by different Mycobacterium tuberculosis genotypes. Clin Exp Immunol. 2003;133(1):30-7.

3. Barczak AK, Domenech P, Boshoff HI, Reed MB, Manca C, Kaplan G, et al. In vivo phenotypic dominance in mouse mixed infections with Mycobacterium tuberculosis clinical isolates. J Infect Dis. 2005;192(4):600-6.

4. Canetti G, Rist N, Grosset J. Measurement of sensitivity of the tuberculous bacillus to antibacillary drugs by the method of proportions. Methodology, resistance criteria, results and interpretation [Article in French]. Rev Tuberc Pneumol (Paris). 1963;27:217-72.

5. van Embden JD, Cave MD, Crawford JT, Dale JW, Eisenach KD, Gicquel B, et al. Strain identification of Mycobacterium tuberculosis by DNA fingerprinting: recommendations for a standardized methodology. J Clin Microbiol. 1993;31(2):406-9.

6. Saad MH, Fonseca LD, Ferrazoli L, Fandinho F, Palaci M, Grinsztejn B, et al. IS1245 genotypic analysis of Mycobacterium avium isolates from patients in Brazil. Int J Infect Dis. 1999;3(4):192-6.

7. Tavares RC, Salgado J, Moreira VB, Ferreira MA, Mello FC, Leung JW, et al. Interferon gamma response to combinations 38 kDa/CFP-10, 38 kDa/MPT-64, ESAT-6/MPT-64 and ESAT-6/CFP-10, each related to a single recombinant protein of Mycobacterium tuberculosis in individuals from tuberculosis endemic areas. Microbiol Immunol. 2007;51(3):289-96.

8. Ordway D, Palanisamy G, Henao-Tamayo M, Smith EE, Shanley C, Orme IM, et al. The cellular immune response to Mycobacterium tuberculosis infection in the guinea pig. J Immunol. 2007;179(4):2532-41.

9. Valway SE, Sanchez MP, Shinnick TF, Orme I, Agerton T, Hoy D, et al. An outbreak involving extensive transmission of a virulent strain of Mycobacterium tuberculosis. N Engl J Med. 1998;338(10):633-9. Erratum in: N Engl J Med 1998;338(24):1783.

10. Manca C, Tsenova L, Barry CE 3rd, Bergtold A, Freeman S, Haslett PA, et al. Mycobacterium Tuberculosis Cdc1551 Induces A More Vigorous Host Response In Vivo And In Vitro, But Is Not More Virulent Than Other Clinical Isolates. J Immunol. 1999;162(11):6740-6.

11. Sharma MK, Al-Azem A, Wolfe J, Hershfield E, Kabani A. Identification of a predominant isolate of Mycobacterium tuberculosis using molecular and clinical epidemiology tools and in vitro cytokine responses. BMC Infect Dis. 2003;3:3.

12. McDyer JF, Hackley MN, Walsh TE, Cook JL, Seder RA. Patients with multidrug-resistant tuberculosis with low CD4+ T cell counts have impaired Th1 responses. J Immunol. 1997;158(1):492-500.

13. Fortes A, Pereira K, Antas PR, Franken CL, Dalcolmo M, Ribeiro-Carvalho MM, et al. Detection of in vitro interferon-gamma and serum tumour necrosis factor-alpha in multidrug-resistant tuberculosis patients. Clin Exp Immunol. 2005;141(3):541-8.



* Study carried out in the Laboratory of Cellular Microbiology. Fundação Instituto Oswaldo Cruz - Fiocruz, Oswaldo Cruz Institute Foundation - Rio de Janeiro, Brazil.
Correspondence to: Maria Helena Féres Saad. Laboratório de Microbiologia Celular, Instituto Oswaldo Cruz, Fiocruz, Avenida Brasil, 4365, CEP 21045-900, Rio de Janeiro, RJ, Brasil.
Tel 55 21 2598-4346. Fax 55 21 2270-9997. E-mail: saad@ioc.fiocruz.br
Financial support: The study received financial support from the Conselho Nacional de Desenvolvimento Científico e Tecnológico (CNPq, National Council for Scientific and Technological Development; grant number 573548/2008-0 and 470558/2008-3) and from the Fundação de Amparo a Pesquisa do Estado do Rio de Janeiro (FAPERJ, Foundation for the Support of Research in the State of Rio de Janeiro; grant E-26/111657/2008).
Submitted: 20 January 2010. Accepted, after review, 17 March 2010.
** A versão completa em português deste artigo está disponível em www.jornaldepneumologia.com.br



About the authors

Vinícius Ribeiro Cabral
Biologist. Laboratory of Cellular Microbiology. Fundação Instituto Oswaldo Cruz - Fiocruz, Oswaldo Cruz Institute Foundation - Rio de Janeiro, Brazil.

Cláudia Ferreira de Souza
Biologist. Laboratory of Cellular Microbiology. Fundação Instituto Oswaldo Cruz - Fiocruz, Oswaldo Cruz Institute Foundation - Rio de Janeiro, Brazil.

Fernanda Luiza Pedrosa Guimarães
Biologist. Laboratory of Cellular Microbiology. Fundação Instituto Oswaldo Cruz - Fiocruz, Oswaldo Cruz Institute Foundation - Rio de Janeiro, Brazil.

Maria Helena Feres Saad
Lead Researcher. Laboratory of Cellular Microbiology. Fundação Instituto Oswaldo Cruz - Fiocruz, Oswaldo Cruz Institute Foundation - Rio de Janeiro, Brazil.

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