INTRODUCTION
Non-tuberculous mycobacteria (NTM) are opportunistic pathogens causing mycobacteriosis in humans and animals. The members of Mycobacterium avium complex (MAC) are the most frequent etiological agents of mycobacteriosis and differ in the type of disease they cause and their pathogenicity [Reference Karakousis, Moore and Chaisson1–Reference Falkingham3].
M. avium subsp. paratuberculosis (MAP) causes paratuberculosis in ruminant animals [Reference Whittington and Windsor4], and it has been postulated that MAP could also have a potential zoonotic role as it has been isolated from patients with Crohn's disease [Reference Sechi5, Reference El-Zaatari, Osato and Graham6]. The other MAC members have no primary host animal and they can be found in the environment as free-living organisms [Reference Vaerewijck7, Reference Falkinham8].
M. avium, the main MAC mycobacteria, is a heterogeneous group of four subspecies. Identification is based on molecular typing by different genomic targets, including the presence and distribution of several insertion sequences (IS) [Reference Rindi and Garzelli9, Reference Motiwala10]. The four subspecies of M. avium are: (a) MAP that contains IS900 [Reference Vaerewijck7]; (b) M. avium subsp. avium (MAA), which contains IS901 and could affect humans [Reference Bruijnesteijn11–Reference Barandiarán14]; (c) MAS (M. avium subsp. silvaticum) that also has IS901 [Reference Thorel, Krichevsky and Lévy-Frébault15]; and (d) M. avium subsp. hominissuis (MAH), the leading member of the MAC causing disseminated or pulmonary disease in humans.
MAH can also produce mycobacterioses in pigs [Reference Inderlied, Kemper and Bermudez16] and could be a source of M. avium transmission to humans [Reference Lara13, Reference Barandiarán14, Reference Johansen17, Reference Pate18]. In fact, there were isolated MAH strains from humans and pigs sharing identical or closely similar genotypes and, while this does not confirm the potential zoonotic role of this subspecies, it cannot be ruled out either [Reference Rindi and Garzelli9, Reference Möbius19, Reference Mijs20].
Remarkably the IS1311 is present in the four M. avium subspecies [Reference Johansen21] and contains polymorphisms (point mutations) useful to distinguish it from the other subspecies [Reference Whittington22].
Molecular techniques based on the polymorphisms present in the length of fragments obtained by restriction enzymes [Restriction fragment length polymorphism (RFLP)] of specific IS (IS900, IS1245, and IS1311) have been used to differentiate MAC subspecies and even strains belonging to the same subspecies [Reference Motiwala10, Reference Radomski23]. This method, however, is very laborious and requires large amounts of genomic DNA seldom obtained from MAP [Reference Travería24].
Polymerase chain reaction and restriction endonuclease analysis (PCR–REA) (restriction fragment analysis) of the IS1311 allowed the differentiation between two major MAP lineages (type S, sheep type and type C, cattle type). The strain types were extended to types I and III (subtypes of type S), and type II (subtype of type C) and strains isolated from Bison species [Reference Bryant25].
A PCR-based molecular typing method (based on mycobacteria repetitive elements) called mycobacterial interspersed repetitive-unit-variable-number tandem-repeats (MIRU-VNTRs) has been used for genotyping different mycobacteria species [Reference Radomski23, Reference Sola26–Reference Iakhiaeva28]. Thibault et al. (2007) applied a MIRU-VNTR scheme using eight MIRU-VNTR loci (MIRU 292, MIRU X3, VNTR 25, VNTR 47, VNTR 3, VNTR 7, VNTR 10, and VNTR 32) for genotyping MAP isolates. The high discriminatory index (DI: 0·751) made it possible to apply this technique to other MAC members [Reference Radomski23, Reference Thibault29].
In this study, we aimed to describe the genetic diversity of MAC, from human and animal origins, causing disease in different hosts in Argentina.
METHODS
MAC isolates
M. avium isolates
M. avium isolates from humans were obtained from the Reference Laboratory of Tuberculosis Control Programme at Dr Antonio A. Cetrangolo Hospital where the patients had received medical attention. The study period was from April 2010 to December 2015. To obtain M. avium isolates, pulmonary, and extra-pulmonary specimens were homogenized and decontaminated using a mixture of NaCl/NaOH [Reference Morcillo, Imperiale and Palomino30]. The mycobacterial isolates from both pulmonary and extra-pulmonary specimens were obtained in Löwenstein–Jensen, Stonebrink and MGIT960™ (BD, Argentina) with the only exception of blood and bone marrow samples that were inoculated in the Myco-F-Lytyc bottles for their incubation in the Bactec 9050™ system (BD).
MAP isolates
MAP isolates were obtained at the Veterinary Research Center (CEDIVE-National University of La Plata (UNLP)) from stool and/or intestinal mucosa from cattle. Clinical samples were homogenized and decontaminated by the HPC (hexadecylpyridinium chloride) method [Reference Ikonomopoulos31] and loaded into Herrolds, M7H10/OADC and M7H9/OADC media supplemented with mycobactin J (2 mg/l) and incubated at 37°C for at least 4 months.
Geographic distribution
All patients affected by MAC came from the 5th Sanitary Region of Buenos Aires Province, which covers a surface of approximately 30 000 km2, with 13 districts and municipalities distributed in either rural or urban areas with 3·131·892 inhabitants. MAP isolates came from different locations of Buenos Aires Province such as Tandil, Chascomús, Bartolomé Bavio, Vieytes, Lomas de Zamora. Figure 1 shows the geographical region of the isolates.
Identification of mycobacterial species
When microbial development was observed in culture media, the presence of acid-fast bacilli was confirmed by Ziehl–Neelsen stain. PCR of specific IS (IS900, IS1311, IS901) was performed for species identification and/or through GenoType CM™ (human isolates) [Reference Collins, Cavaignac and de Lisle32, Reference Marsh, Whittington and Cousins33].
Characterization of MAC subspecies by IS1311 PCR–REA
The identified MAC subspecies were characterized using restriction enzymes according to the polymorphism present in position 223 of the IS1311. The IS1311 PCR product was digested by HinfI and MseI [Reference Marsh, Whittington and Cousins33].
Genotyping of MAC isolates by MIRU-VNTR assay
Genotyping of MAC isolates using this system included the amplification of eight MIRU-VNTR loci (292, X3, 25, 47, 3, 7, 10, 32) previously reported by Thibault et al. [Reference Thibault29]. Primers used to amplify each locus were as previously reported [Reference Thibault29]. The amplification protocol was modified to amplify the eight loci simultaneously using touchdown programme at 95°C for 3 min, nine cycles of 95°C for 30 s, 62°C (−0·5°/cycle) for 30 s, and 72°C for 30 s; followed by 30 cycles at 95°C for 30 s, 58°C for 30 s, and 72°C for 30 s with a final extension at 72°C for 7 min. The Mix protocol included 1·5 mM MgCl2, 2 µl DMSO, 1·25 U Taq, 2 mM dNTPs mix, and different amounts of primers (from 10 to 25 pmol according to the locus to be amplified). To determine the molecular weight (MW) of each PCR product and to estimate the number of tandem repeats present in each loci, 10 µl of PCR product were loaded in a 2% agarose gel. MW markers (50 and 100 bp) were included on the gel. To digitalize the gel the Gel Doc TM imager (Bio-Rad) was used and the results were expressed by an octal code and the genotype pattern (INMV) was determined using the international online MAC-INMV database (http://mac-inmv.tours.inra.fr/index.php?p=nomenclature).
Discriminatory power
The allelic diversity (D) of each MIRU-VNTR locus and the global discriminatory power of complete MIRU-VNTR scheme (HGDI) were determined using the Hunter and Gaston discriminatory index [Reference Hunter34, Reference Hunter and Gaston35].
where N is the total number of isolates in the typing scheme, s is the total number of distinct subtypes discriminated by the typing method, and xj is the number of isolates belonging to the xth subtype.
The index (D and HGDI) were calculated using the online software http://insilico.ehu.es/mini_tools/discriminatory_power/, University of the Basque Country.
The relation among the different INMV profiles was presented in a dendrogram and probable patterns of evolutionary descent between allelic profiles (clonal relationship) was inferred using the goeBURST algorithm, through the Minimum Spanning Tree (MST). It is assumed that the genetic distance between two INMV patterns, is proportional to the difference in the number of repeats at each locus. These relations were established using Phyloviz 2 software (http://goeburst.phyloviz.net) [Reference Francisco36].
RESULTS
MAC isolates
Human isolates
Of 31 M. avium isolates that were obtained from human samples at Dr Antonio A. Cetrangolo Hospital, they were identified at species level, by GenoType CM (Hain Lifescience), as M. avium I (n: 20), M. avium II (n: 6), and M. intracellulare (n: 5). The IS1311 PCR was positive for the 26 isolates classified as M. avium I or II by GenoType. The 26 isolates were analyzed by PCR for IS901 and all were found to be negative, confirming that the isolates belonged to MAH and also confirming the absence of MAA among the studied isolates.
Isolates from cattle
A total of 61 isolates obtained from cattle at CEDIVE, were confirmed as MAC by IS1311 PCR and as MAP by IS900 PCR.
Characterization of MAC subspecies by IS1311 PCR–REA
All MAC isolates were classified according to the polymorphism at the position 223 present in the IS1311, by PCR–REA. The restriction pattern obtained after digestion with HinfI (323, 285, 218, and 67 bp) allowed us to identify the most prevalent type of MAP (type II/C or cattle type) among the 61 isolates. As expected, due to the difficulty of culturing type S isolates and their host preference for sheep or goats, no type S/type I/III isolates (with restriction fragments of 285 and 323 bp) were found among the isolates in this study. The 26 MAH isolates showed three restriction bands (134, 189, and 285 bp). Additionally, restriction with MseI allowed discrimination between MAH and MAP (no restriction of MAP).
Genotyping of MAC isolates by MIRU-VNTR assay
A total of 83 out of 87 (95·4%) MAC was successfully genotyped.
MAH isolates
A total of 84·6% (n: 22/26) of MAH isolates showed results. Sixteen isolates were grouped among five different previously described INMV patterns (INMV 92, n: 4; INMV 121, n: 4; INMV 97, n: 2; INMV 103, n: 2; INMV 50, n: 2 and INMV 40, n: 2). Six MAH isolates showed novel patterns (NC1, NC2, NC3, NC4, NC5, and NC6) that we reported to National Institute for Agricultural Research and incorporated into the MAC-INMV database. They were assigned to different INMV numbers: 144 (NC1), 145 (NC2), 146 (NC3), 147 (NC4), 148 (NC5), and 149 (NC6). Another four MAH isolates had an incomplete genotyping profile (Table 1). This system showed a high discriminatory power (HGDI: 0·930) for MAH isolates. With regards the discriminatory power (D) of each locus, the loci X3 and 25 showed the higher D value (D: 0·5844), followed by locus 292 (D: 0·5714), locus7 (D: 0·4848), locus 47 (D: 0·3247), locus 10 (D: 0·2554). Loci 3 and 32 did not show allelic diversity (D: 0·0909 and D: 0, respectively).
TR, number of tandem repeats in each locus; MIRU-VNTR, mycobacterial interspersed repetitive-unit-variable-number tandem-repeat; NC, unknown pattern that were recently assigned in the MAC-INMV database with an INMV number; IP, incomplete profile; MAP, Mycobacterium avium sp. paratuberculosis; MAH, M. avium sp. hominissuis; CABA, autonomous city of buenos aires; S/D, unknown.
MAP isolates
The totality of the isolates (100%) were genotyped and grouped into five different INMV previously reported patterns (24, 30). INMV 1 and INMV 2 were the patterns most frequently found (INMV 1, 44·2% and INMV 2, 27·9%), followed by INMV 11 (21·3%), INMV 8 (3·3%), and INMV 5 (3·3%). This technique when applied to MAP showed a lower discriminatory index (HGDI: 0·6984) than that obtained for MAH isolates. Loci 7 and 292 had higher allelic diversities (D: 0·6980 and 0·5050, respectively), locus 10 a low D (0·0645) while loci X3, 25, 47, 3, and 32 showed no variability.
Relation between isolates
The relation between the different MAC isolates is shown in a dendrogram (Fig. 2) and the clonal relationship between the isolates was calculated using the goeBURST algorithm through the MST (Figs 3 and 4). Figure 3 indicates the INMV 2 of MAP as the original clone from which the others derive. The clonal relationship obtained by goeBURST algorithm including our MAH and MAP isolates, showed two INMV MAH genotypes (NC5: INMV148 and NC6: INMV 149) that were not previously reported and were very closely related to the INMV 2 of MAP that is the original clone from which MAP clones originate. In the case of MAH, clones 92 and 97 are the originals from which all other MAH clones originate. In addition, in Figure 3, it is observed that the unknown patterns of MAH NC5 (INMV 148) and NC6 (INMV 149) originated from INMV 2 of MAP. However, these isolates were negative for IS900 (data not shown). Interestingly, when our isolates were analyzed in a global context including all the INMV patterns previously reported in the international online MAC-INMV database, it was observed that the patterns NC5 (INMV 148) and NC6 (INMV 149) were grouped with the MAH isolates.
Geographic distribution
While, both MAP and MAC isolates were obtained from Buenos Aires Province, the geographical region of MAH isolates was smaller when compared with the MAP region; however, MAH isolates showed greater genetic variability when compared with the MAP isolates. Table 1 summarizes the different INMV patterns found distributed by geographical area for both MAH and MAP.
DISCUSSION
PCR-based methods have simplified genotyping of microorganisms and in particular the MIRU-VNTR was easy to perform and required a low quantity of DNA. This technique was useful to describe the genetic diversity present among the MAH and MAP isolates studied. MAH showed a higher genetic diversity than MAP, indicating that using only MIRU-VNTR was sufficient for genotyping MAH isolates and to describe the genetic diversity of their subspecies. On the other hand, an acceptable HGDI was obtained for MAP, and was in agreement with those reported by other authors [Reference Radomski23, Reference Gioffré37].
Since the INMV patterns obtained from the study could be compared with those reported in a free MAC-INMV database (http://mac-inmv.tours.inra.fr/), the eight MIRU-VNTR loci scheme was therefore performed. Six patterns were described for the first time in this study and, following reporting, were subsequently included in the database.
In addition, we identified two unknown MAC-INMV patterns (NC5 and NC6) that were grouped within other MAH isolates by MST when all the MAH strains previously reported in the database were included in the analysis (Fig. 4).
In accordance with the D value obtained for each locus of the loci and the global HGDI, a shortened scheme could be used for genotyping MAP isolates. This scheme could include only the loci 7, 292, 10, and 25. Additionally, it has been reported that the use of MIRU-VNTR combined with a second method, such as the polymorphisms present in multilocus short sequence repeats (MLSSR) improve the genotyping approach for high-resolution typing of MAP due to their additive discriminatory power [Reference Amonsin38, Reference Thibault39]. The addition of another genotyping technique using different discriminatory genetic markers could improve the classification of isolates. An example includes where studies assessed the genetic relationship of MAP isolates using whole genome sequencing (WGS) and VNTR typing. The studies reported that VNTR typing may lead to an incorrect assessment of diversity and origins of strains. A weakness of this study was that using VNTR genotyping techniques you may either overestimate or underestimate the relationship between strains due to the instability of some repetitive elements in the genome and the occurrence of homoplasy [Reference Francisco40]. Homoplasy is the occurrence of genotypes that are identical by state but not by descent and can be originated by horizontal gene transfer and by convergent and reverse evolution [Reference Bryant25, Reference Ahlstrom41].
The main patterns found among the studied MAP isolates were INMV 1 and 2. These findings were in agreement with those previously reported as the most prevalent in different parts of the world [Reference Thibault29, Reference Gioffré37]. The prevalence reported by the MAC-INMV database for the most common patterns were INMV 1: 27·92% and INMV 2: 23·71% (http://mac-inmv.tours.inra.fr/index.php?p=fa_db).
With regards MAH isolates, INMV 92 and 121 were the most prevalent patterns among our isolates, but they were not reported as the most frequent genotypes of MAH on the database. Interestingly, INMV 92 was found only in one district (Escobar) of the Sanitary Region V of Buenos Aires Province (Fig. 1).
A limitation of this study was that not all MAC subspecies were represented among the isolates studied, although MAH and MAP are the main subspecies of the complex causing disease in humans and animals, respectively.
In this study it was demonstrated that mycobacterioses caused by MAC in humans were produced mainly by MAH, as no MAA clinical isolates were found among the human clinical samples. On the other hand, previous studies carried out also in Buenos Aires Province, but not in the exact region of this study, reported mycobacterioses in pigs caused by MAC. In that study, most of the cases were caused by MAA (n: 30) instead of MAH (n: 6) [Reference Barandiarán14]. However, although it has been postulated the possible zoonotic role of MAH, the INMV patterns found for MAH isolates from pigs in Buenos Aires Province, were different from those found in the present study [Reference Barandiarán14].
The strength of this study was mainly represented by the simplicity and usefulness of the MIRU-VNTR technique and the facilitated analysis on the diversity of strains. In addition, while previous work performed in Argentina showed the distribution of MAP patterns in different host and regions from Buenos Aires Province [Reference Gioffré37], to the best of our knowledge no previous reports exist to date about the genetic diversity of other MAH members in this country by MIRU-VNTR typing. However, further studies, including more clinical and cattle samples, could contribute to increasing the knowledge of the genotypic diversity of these organisms in addition to exclude or not the MAA as a human pathogen.
ACKNOWLEDGMENTS
B.R. Imperiale, M.P. Santangelo and M.I. Romano are fellows of CONICET. R.D. Moyano has a fellowship from CONICET. The authors thank Dr. Barry James Cole from BMS (Bristol-Myers Squibb), Swords Laboratories, Ireland, for their English technical support. He has reviewed the entire manuscript.
DECLARATION OF INTEREST
None.