Differentiation of tuberculosis strains in a population with mainly Beijing-family strains.A high prevalence of tuberculosis (TB) isolates that are genetically homogenous homogenous - homogeneous and from the Beijing family has been reported in Russia. To map TB transmission caused by these strains, new genotyping Genotyping refers to the process of determining the genotype of an individual with a biological assay. Current methods of doing this include PCR, DNA sequencing, and hybridization to DNA microarrays or beads. systems are needed. Mycobacterial mycobacterial emanating from or pertaining to mycobacterium. mycobacterial granuloma may be caused by Mycobacterium tuberculosis (see cutaneous tuberculosis), M. interspersed repetitive units (MIRUs) offer the possibility of rapid PCR-based typing with comparable discrimination to IS6110 restriction fragment length polymorphism restriction fragment length polymorphism n. Abbr. RFLP Intraspecies variations in the length of DNA fragments generated by the action of restriction enzymes and caused by mutations that alter the sites at which these enzymes act, changing techniques. Spoligotyping and detection of IS6110 insertion in the dnaA-dnaN region were used to identify Beijing strains in 187 Mycobacterium tuberculosis Mycobacterium tuberculosis n. Tubercic bacillus. Mycobacterium tuberculosis isolates from Samara, Russia This article is about the city in Russia. For the city in Iraq, see Samarra Samara (Russian: Сама́ра) (from 1935 to 1991—Kuybyshev ( . The Beijing isolates were analyzed by using 12-MIRU and 3-exact tandem repeats (ETR ETR Estimated Time of Return/Repair ETR Early to Rise (health e-zine) ETR Effective Tax Rate Etr Etruscan (linguistics) ETR Eastern Test Range ETR Express Toll Route ) loci loci [L.] plural of locus. loci Plural of locus, see there and by an expanded set of 10 additional variable number tandem repeats A variable number tandem repeats (VNTR) is a short nucleotide sequence ranging from 14 to 100 nucleotides long that is organized into clusters of tandem repeats, usually repeated in the range of between 4 and 40 times per occurrence. loci. The expanded set of 25 MIRUs provided better discrimination than the original set of 15 (Hunter-Gaston diversity index 0.870 vs 0.625). Loci MIRU MIRU Move In Rig Up MIRU Magnetohydrodynamic Inertial Reference Unit MIRU Mycobacterium Interspersed Repetitive Units 26, 1982, and 3232 were the most polymorphic polymorphic - polymorphism in isolates. ********** Rising rates of tuberculosis (TB) (1) and increasing resistance of drugs are substantial barriers to successful patient management and TB control programs. Russia, named by the World Health Organization as one of the 22 countries with the highest TB prevalence, has seen increasing rates of TB and HIV HIV (Human Immunodeficiency Virus), either of two closely related retroviruses that invade T-helper lymphocytes and are responsible for AIDS. There are two types of HIV: HIV-1 and HIV-2. HIV-1 is responsible for the vast majority of AIDS in the United States. during the past decade (2-6) and high levels of resistance, particularly to multiple drugs (7,8). The high discriminatory power of restriction fragment length polymorphism (RFLP RFLP abbr. restriction fragment length polymorphism RFLP restriction fragment length polymorphism. RFLP ) analysis based on the insertion sequence insertion sequence n. Any of several discrete DNA sequences that repeat at various sites on a bacterial chromosome, on certain plasmids, and on bacteriophages and that can move from one site to another on the chromosome, to another plasmid in the same IS6110 has provided the backbone of these analyses (9). Unfortunately, the technique is time-consuming, technically demanding, and insufficiently discriminating when used alone with isolates containing <5 IS6110 sequences in the genome (10,11). Isolates with low numbers of copies account for as much as 20% of TB isolates in some populations (12). Techniques based on PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) amplification of repetitive sequences are more rapid than RFLP, but their discriminatory power is usually lower. Among these techniques, spoligotyping is widely used to differentiate strains belonging to the Mycobacterium tuberculosis complex. Spoligotyping has been particularly useful for identifying strains belonging to the Beijing/W family of M. tuberculosis M. tuberculosis, n the bacterium responsible for tuberculosis, generally a respiratory infection in man; nonrespiratory tuberculosis is considered an indicator disease for AIDS. See also tuberculosis. because of the characteristic spoligotyping pattern with the absence of spacers 1-34 in the direct repeat (DR) region of the M. tuberculosis genome (13). Beijing family strains are dominant across many Asian and former Soviet Union countries, and W strains are responsible for outbreaks of multidrug-resistant TB in the United States United States, officially United States of America, republic (2005 est. pop. 295,734,000), 3,539,227 sq mi (9,166,598 sq km), North America. The United States is the world's third largest country in population and the fourth largest country in area. . These strains are now considered to be members of the same phylogenetic phy·lo·ge·net·ic adj. 1. Of or relating to phylogeny or phylogenetics. 2. Relating to or based on evolutionary development or history. lineage, sharing key characteristics such as a similar RFLP pattern of 15-26 bands, IS6110 insertions in the dnaA-dnaN and NTF-1 chromosomal regions, a characteristic pattern of single nucleotide polymorphism Noun 1. single nucleotide polymorphism - (genetics) genetic variation in a DNA sequence that occurs when a single nucleotide in a genome is altered; SNPs are usually considered to be point mutations that have been evolutionarily successful enough to recur in a , and a spoligotyping pattern with the presence of spacers 35-43 and absence of spacers 1-34 in the DR region of the M. tuberculosis genome (14-17). Detecting the IS6110 insertion in the dnaA-dnaN intergenic region An Intergenic region is a stretch of DNA sequences located between clusters of genes that comprise a large percentage of the human genome but contain few or no genes. Occasionally some intergenic DNA acts to control genes close by, but most of it has no currently known function. may also identify the Beijing/W genotype genotype (jēn`ətīp'): see genetics. genotype Genetic makeup of an organism. The genotype determines the hereditary potentials and limitations of an individual. (14,15). Several studies have shown that a high proportion of TB isolates in Russia (particularly those that are drug resistant) belong to the Beijing family (7,8,18). To assess TB transmission in Russia, any genotyping system must be able to discriminate among Beijing strains. The identification of variable number tandem repeats (VNTRs) (19) in M. tuberculosis has offered the possibility of rapid amplification-based techniques with comparable discrimination to RFLP-IS6110 typing (20-23). As with other PCR-based genotyping techniques, VNTR VNTR Variable Number of Tandem Repeat(s) analysis uses small quantities of crude bacterial lysates; it is less labor-intensive than RFLP-IS6110 typing, and automation is relatively straightforward (22). Moreover, determination of a limited number of polymorphic loci can provide sufficient discriminative dis·crim·i·na·tive adj. 1. Drawing distinctions. 2. Marked by or showing prejudice: discriminative hiring practices. power for a given local population and may increase the cost-effectiveness of molecular typing. Several panels of M. tuberculosis VNTRs have been used with some success previously: exact tandem repeats (ETRs) (19), MIRUs (21,22), and 2 panels of loci known as QUB QUB Queen's University Belfast QUB Q Universal Boardgame QUB Weather Report (radiotelegraphy) and Mtub (24-27). Our aim was to determine the discriminative power of an expanded set of 25 VNTR loci when applied to TB strains in Russia where Beijing strains dominate. Methods M. tuberculosis Strains A total of 187 M. tuberculosis strains were analyzed. They were selected from 880 M. tuberculosis strains isolated from patients (1 isolate per patient) with radiologically confirmed pulmonary TB pulmonary TB Pulmonary tuberculosis, see there , identified from all TB treatment facilities across Samara Oblast Samara Oblast (Russian: Сама́рская о́бласть, Samarskaya oblast) is a federal subject of Russia (an oblast). in central Russia (12 civilian TB hospitals and dispensaries and 1 prison TB hospital) during 2001-2002. The test panel included 138 (33.7%) of 409 strains isolated from patients in the civilian TB hospitals and dispensaries and 49 (10.4%) of 471 isolates from prisoners. Within sets of cultures isolated from civilians, every third isolate was selected for this study. Because isolates from prisoners were overrepresented o·ver·rep·re·sent·ed adj. Represented in excessive or disproportionately large numbers: "Some groups, and most notably some races, may be overrepresented and others may be underrepresented" , every 10th isolate was selected. The representation of isolates in the test panel was approximately proportional to the number of TB isolates from each clinical site. In the Samara Samara, river, Russia Samara (səmä`rə), river, c.360 mi (580 km) long, rising in the foothills of the S Urals, European Russia. It flows generally northwest, and joins the Volga River at Samara. region, the incidence of TB at the time of the study was 86.1/100,000 population. Patient populations are described in previous publications (18,28). All patients with TB are tested for HIV as a part of routine practice in Russia. History of vaccination with M. bovis BCG BCG bacille Calmette-Guérin. BCG abbr. 1. bacillus Calmette-Guérin 2. ballistocardiogram BCG, n.pr See bacille Calmette-Guórin. was confirmed by presence of an appropriate scar. Molecular Epidemiologic Analysis Crude DNA DNA: see nucleic acid. DNA or deoxyribonucleic acid One of two types of nucleic acid (the other is RNA); a complex organic compound found in all living cells and many viruses. It is the chemical substance of genes. extracts were obtained by heating cell suspensions with chloroform chloroform (klôr`əfôrm) or trichloromethane (trī'klôrōmĕth`ān), CHCl3 at 80[degrees]C as previously described (29). Spoligotyping used a standardized method (30) to identify isolates belonging to the Beijing family; results were confirmed by analysis of the dnaA to dnaN region in all isolates. The IS6110 insertion in the origin of replication The origin of replication (also called the replication origin) is a particular DNA sequence at which DNA replication is initiated. DNA replication may proceed from this point bidirectionally or unidirectionally. was detected between dnaA and dnaN genes as described previously (15,16). Briefly, PCR was performed in a 20-[micro]L volume of 2 [micro]L 10x PCR buffer (Bioline Ltd, London, UK); 0.5 units Taq polymerase Taq polymerase ("Taq Pol," or simply "Taq") is a thermostable polymerase used in polymerase chain reaction to check for the presence or absence of a gene by amplifying a DNA fragment. It replaced E.coli DNA polymerase in PCR because of the temperature conditions of PCR. (Bioline Ltd); 0.5 [micro]L 2 mmol dNTP mixture (Bioline Ltd); 0.5 [micro]L 20-[micro]mol mix of forward and reverse primers, 15.5 [micro]L water, and 1 [micro]L of crude DNA extract. Thermal cycling was performed on a PerkinElmer 9700 thermocycler (PerkinElmer, Warrington, UK) as follows: 4 min at 94[degrees]C; 30 cycles of 30 s at 94[degrees]C, 30 s at 60[degrees]C, and 2 min at 72[degrees]C; followed by 7 min at 72[degrees]C and holding at 4[degrees]C. Amplification products were analyzed by electrophoresis on 1.5% agarose agarose more highly purified form of agar with similar uses to agar and widely used in the separation of nucleic acid fragments. gel. Strains with insertion (i.e., Beijing family) yielded a product of [approximately equal to] 2 kb, and fragments of [approximately equal to] 550 bp (no insertion) indicated strains other than Beijing. All 187 TB isolates were tested by using the set of 12-MIRU loci and the 3-ETR (A, B, and C) loci (19,22) (nos. 1-15, online Appendix Table, available from http://www.cdc.gov/ncidod/EID/vol12no09/04-1263_appT.htm). Beijing isolates were further analyzed by using an additional panel of VNTR loci (0424, 0531, 1955, 1982, 2074, 2163a, 3232, 3239, 3336, and 3690, online Appendix Table). Primers for loci at which predicted fragment size would exceed 1 kb were redesigned to enable analysis with the CEQ CEQ Council On Environmental Quality CEQ Course Experience Questionnaire (higher education) CEQ Centrale de l'Enseignement du Québec CEQ Cinema Equalizer 8000 equipment (Beckman Coulter This article needs sources or references that appear in reliable, third-party publications. Alone, primary sources and sources affiliated with the subject of this article are not sufficient for an accurate encyclopedia article. , Fullerton, CA, USA). Multiplex See multiplexing. and simplex PCRs were performed, taking into consideration dye labeling and expected length of PCR products. Simplex PCR was used to amplify fragments in loci MIRU 20, ETR-C, MIRU 26, VNTR 424, VNTR 531, VNTR 1955, VNTR 1982, VNTR 2163a, VNTR 3232, VNTR 3239, and VNTR 3336. For other loci, multiplex PCR mixtures were prepared as follows: set 1 contained MIRU 4 and MIRU 16, set 2 contained MIRU 39 and ETR-A, set 3 contained MIRU 2 and MIRU 24, set 4 contained MIRU 31 and MIRU 40, set 5 contained MIRU 10 and MIRU 23, set 6 contained MIRU 27 and ETR-B, and set 7 contained VNTR 2074 and VNTR 3690. For all mixtures, PCR was performed in 10-[micro]L volumes containing 1 [micro]L 10x PCR buffer (containing 1.5 mmol/L Mg[Cl.sub.2], Bioline Ltd); 0.5 U Taq polymerase (Bioline Ltd); 0.25 [micro]l 2-mmol dNTP mixture (Bioline Ltd); 0.5 [micro]L 20-[micro]mol mixture of forward and reverse primers as described above, 7.0 [micro]L water, and 1 [micro]L DNA extract. For loci VNTR 424, VNTR 531, VNTR 1955, VNTR 1982, VNTR 2074, VNTR 2163a, VNTR 3232, VNTR 3239, VNTR 3336, and VNTR 3690, the mixture also contained 0.5 [micro]L dimethylsulfoxide di·meth·yl·sulf·ox·ide n. DMSO. (Sigma, Dorset, UK). Thermal cycling programs were identical for all loci, and thermal cycling was performed on a PerkinElmer 9700 thermocycler by using the following parameters: 3 min at 95[degrees]C; 30 cycles of 30 s at 95[degrees]C, 30 s at 60[degrees]C, and 60 s at 72[degrees]C; followed by 5 min at 72[degrees]C. Automated analysis of PCR fragments length was performed by using a Beckman Coulter CEQ8000 automatic sequencer See MIDI sequencer. (music) sequencer - Any system for recording and/or playback of music via a programmable memory which stores music not as audio data, but as some representation of notes. . Multiple PCR products were analyzed in capillaries as follows: capillary 1 contained PCR products for loci 2, 4, 10, 16, 23, and 24; capillary 2 for loci 27, 31, 39, ETR-A, and ETR-B; capillary 3 for loci 20, 26, and ETR-C; capillary 4 for loci 0424, 0531, and 1955; capillary 5 for loci 2974, 3232, 3239, and 3690; and capillary 6 for loci 1982, 2163a, and 3336. Before being loaded onto the sequencer, PCR products were diluted in purified water Purified water can come from any source, including spring water, well water, seawater, or municipal water. This source water is then processed by reverse osmosis or deionization to produce a water that is indistinguishable from distilled water from any other source. (Sigma) as follows: products labeled with dye 2 were diluted to 10-fold; with dye 3, to 30-fold; and with dye 4, to 60-fold. A total of 1 [micro]L of diluted PCR products mixture was added to 25 [micro]L formamide (Beckman Coulter) containing 0.1 [micro]L of DNA size standard 600 (Beckman Coulter), and 0.1 [micro]L DNA size standard 640-1,000 (Bio Ventures Inc., Murfreesboro, TN, USA), labeled with dye 1. Fragment length estimation was performed by using proprietary software (Beckman Coulter). Molecular weights of PCR-generated fragments for loci 1982 and 3232 for some isolates exceeded 1 kb, and results of automated fragment analysis were inconsistent. Molecular weights of PCR products and numbers of MIRU repeats for these strains were determined manually by electrophoresis on a 1.2% agarose gel (Agarose 1000, Invitrogen Ltd, Paisley, UK) with a 100-bp step DNA ladder A DNA ladder is a solution of DNA molecules of different lengths used in agarose gel electrophoresis. It is applied to an agarose gel as a reference to estimate the size of unknown DNA molecules. as fragment size standard (Promega, Madison, WI, USA) (Figure). [FIGURE OMITTED] Automated calling (in which PCR fragment sizes and allele allele (əlēl`): see genetics. allele Any one of two or more alternative forms of a gene that may occur alternatively at a given site on a chromosome. assignment are automatically determined) or manual determination of genotyping data (number of repeats for each loci) was entered into Microsoft Excel (tool) Microsoft Excel - A spreadsheet program from Microsoft, part of their Microsoft Office suite of productivity tools for Microsoft Windows and Macintosh. Excel is probably the most widely used spreadsheet in the world. Latest version: Excel 97, as of 1997-01-14. (Redmond, WA, USA) tables and imported for further analysis into BioNumerics software (Applied Maths, St Martens, Belgium). Genetic distance analysis and cluster comparison were done by using a categorical variable index and the unweighted pair group method with arithmetic mean (mathematics) arithmetic mean - The mean of a list of N numbers calculated by dividing their sum by N. The arithmetic mean is appropriate for sets of numbers that are added together or that form an arithmetic series. algorithm. If [greater than or equal to] 2 isolates possessed identical VNTR signatures, they were considered to be clustered. For discrimination analysis, Hunter-Gaston diversity index (HGDI) was calculated as described (31) and used for comparison of the discriminatory power of VNTR typing for individual loci and for all loci taken together. Results Baseline clinical and sociodemographic parameters of the 187 TB patients are shown in Table 1. MIRU-ETR analysis of the 187 isolates yielded 10 clusters of indistinguishable isolates and 58 unique patterns. The codes for the 15 loci were expressed in the following order: MIRU 2, 4, 10, 16, 20, 23, 24, 26, 27, 31, 39, 40, ETR-A, ET-RB, ETR-C. Cluster sizes varied from 2 to 75 isolates. The 2 largest clusters consisted of 31 strains with the 223325173533423 profile and 75 strains with the 223325153533423 MIRU-ETR profile, respectively, both consisting of Beijing strains (Table 2). For all strains, genotyping with the 15-MIRU-ETR loci set was more informative and had a higher discriminatory power than with spoligotyping, as expected (HGDI 0.747 for MIRU vs 0.572 for spoligotyping, data not shown). The results of the allelic al·lele n. One member of a pair or series of genes that occupy a specific position on a specific chromosome. [German Allel, short for Allelomorph, allelomorph, from English diversity analysis for all 187 isolates are summarized in Table 3. The discriminatory index for 5 loci (MIRU 26, MIRU 31, MIRU 39, MIRU 40, and ETR-A) exceeded 0.3; these loci were regarded as moderately discriminating according to according to prep. 1. As stated or indicated by; on the authority of: according to historians. 2. In keeping with: according to instructions. 3. definitions proposed in a recent study (23). Other loci were found to be less polymorphic, with HGDIs within the range 0 to 0.3; no polymorphism polymorphism, of minerals, property of crystallizing in two or more distinct forms. Calcium carbonate is dimorphous (two forms), crystallizing as calcite or aragonite. Titanium dioxide is trimorphous; its three forms are brookite, anatase (or octahedrite), and rutile. was registered for loci MIRU 24 and ETR-B. The maximal number of allelic variants (9) was registered for locus MIRU 10, although its discriminatory power was poor because of uneven distribution of isolates with different numbers of repeats. Spoligotyping identified 129 isolates as belonging to the Beijing family (69.0%), a proportion similar to that previously reported for Samara Oblast (7,18). Most (123) of the Beijing isolates had the characteristic spoligotyping profile with 9 final spacers present in the DR region (35-43), whereas 6 isolates had incomplete profiles because they lacked spacer 40 (4 isolates) or 43 (2 isolates). Results of spoligotyping were verified by detection of the IS6110 insertion in the dnaA-dnaN region. All 129 isolates yielded a PCR-product [approximately equal to] 2,000 bp, indicative of Beijing strains. Isolates belonging to strains other then Beijing did not possess an insertion in this region and yielded an [approximately equal to] 550-bp PCR product. The allelic diversity and HGDIs were calculated separately for Beijing strains (Table 4). These were subjected to VNTR analysis by using an additional panel of loci (0424, 0531, 1955, 1982, 2074, 2163a, 3232, 3239, 3336, and 3690; online Appendix Table). The allelic diversity analysis results calculated by using 25-MIRU loci and discriminatory indices are presented in Table 5. Discussion This study evaluated the discriminatory ability of VNTR analysis in a population of patients with TB, in which a predominant proportion of the infecting TB strains belonged to the Beijing family. This genetic group, along with the W family, have been recently shown to share similar characteristics, including absence of spacers 1-34 in the DR region of the M. tuberculosis genome (14,15,17). The latter characteristic, although well known and widely accepted, may not always be definitive for identification of Beijing/W strains alone, as spacers 35-43 are present in several other M. tuberculosis families. Moreover, some spacers (particularly 37, 38, and 40) are missing in certain Beijing/W isolates because of loss of the target for DRa and DRb primers caused by deletions or presence of IS6110 insertions in the DR region (32,33). Results of spoligotyping were confirmed by detection of an IS6110 insertion between the dnaA and dnaN genes, which was found in all 129 Beijing isolates but not in the remaining isolates. Results of our analysis demonstrate 100% specificity of the method and its applicability for robust, rapid, and reliable identification of Beijing family strains. In our study, 6 (4.7%) of 129 isolates identified as Beijing on the basis of spoligotyping had incomplete spoligotyping profiles with a missing spacer 40 or 43. As has been argued by Bifani et al. (32), W strains with missing spacer 40 are defined as W 14 group, characterized by a specific IS6110 RFLP pattern, high levels of drug resistance, and an additional repeat in ETR-D (MIRU 4) locus, i.e., MIRU-ETR profile 23332515 (or 7) 3533423. However, we observed no differences in the number of repeats in the MIRU 4 locus for these 4 isolates. All 4 isolates were multidrug resistant strains. Of the 4 patients, all were male, 1 was HIV-infected, 2 were Russian (1 from Chechnya and 1 from Azerbaijan), and 2 had been vaccinated with BCG. The data from the application of 15-MIRU-ETRs demonstrated the homogeneity and clonality of TB strains in this region of Russia: 135 (72.2%) of 187 strains were clustered into 10 groups, which indicates high rates of recent TB transmission in the Samara region. General trends for VNTR loci diversity and discriminatory power agreed (with some exceptions) with those reported previously (20,22,23,34). The overall allelic polymorphism and discriminatory power of the VNTR loci in this population were lower than that reported in previously published studies because of the large number of Beijing isolates in our test panel. This number reflects the actual prevalence of Beijing strains in Samara Oblast and in the few other regions in Russia for which the proportion of Beijing strains has been described (Tables 2-4). The 15-MIRU-ETR profiles 223325153533423 or 223325173533423 were shared by 106 (82.2%) of the total number of analyzed Beijing strains with an HGDI of 0.625 for all 15 loci. Four loci (MIRU20, MIRU24, MIRU27, and ETR-B) were monomorphic monomorphic /mono·mor·phic/ (-mor´fik) existing in only one form; maintaining the same form throughout all developmental stages. mon·o·mor·phic or mon·o·mor·phous adj. 1. for Beijing strains, and the only locus with sufficient discriminatory power for differentiating among Beijing family strains was MIRU 26. This finding is in marked contrast to the application of MIRU-ETR in other patient populations in which the discriminatory power of MIRU, used in conjunction with spoligotyping, was arguably ar·gu·a·ble adj. 1. Open to argument: an arguable question, still unresolved. 2. That can be argued plausibly; defensible in argument: three arguable points of law. almost comparable to RFLP IS6110 (20-23,35). In these studies, HGDI values were subdivided into 3 groups, according to their ability to discriminate: poor (2, 20, 27), moderate (4, 16, 24, 39, ETR-B, ETR-C), and high (10, 23, 26, 31, 40, ETR-A) (23). We expanded the panel of loci to improve discrimination among the Beijing isolates by using loci that had previously been reported to be highly polymorphic (24-27). The allelic diversity analysis and discriminatory indices are presented in Table 5. The expanded set of VNTRs provided better discrimination than the original set of 15-MIRU-ETRs: 53 different profiles were identified, including 9 shared types in clusters (2-46 isolates each) and 44 unique patterns. The HGDI for 25 VNTR loci together was 0.870 (compared with 0.625 for the original set of MIRU-ETRs). The most discriminatory individual VNTR were loci 3232 and 1982, with a large number of allelic variants (10 and 7, respectively) and HGDIs of 0.621 and 0.489, respectively. Other loci demonstrated poor discriminatory power (HGDI 0-0.2), and locus 2074 was monomorphic. In our analysis of Russian Beijing isolates, 3 loci (MIRU 26, VNTR 1982, and VNTR 3232; 0.3-0.6) were sufficiently polymorphic for differentiation within the Beijing family. A relatively high degree of polymorphism in MIRU 26 has been previously reported (20,23,36). Loci 3232 and 1982 have been much less studied. Locus 3232 was shown to be more polymorphic in M. tuberculosis than in M. bovis (8 vs. 5 allelic variants, respectively) with moderate to high HGDI values (0.60). Locus 3232 displayed the highest discrimination power among 8 novel VNTR loci introduced by Roring et al. (24,25). The basis of polymorphism in loci MIRU 26, VNTR 3232, and VNTR 1982 is not completely clear. The first 2 loci are located in the intergenic regions of genes involved in metabolism of cell membrane Cell membrane The membrane that surrounds the cytoplasm of a cell; it is also called the plasma membrane or, in a more general sense, a unit membrane. This is a very thin, semifluid, sheetlike structure made of four continuous monolayers of molecules. components and transmembrane transmembrane /trans·mem·brane/ (trans-mem´bran) extending across a membrane, usually referring to a protein subunit that is exposed on both sides of a cell membrane. trans·mem·brane adj. transport (locus VNTR 3232) and between genes Rv2679 (possible echA15, enoyl-CoA hydratase Enoyl-CoA hydratase is the enzyme used to catalyze the second step of β-oxidation in Fatty acid metabolism. It catalyzes the following reaction: ) and Rv 2680 (unknown protein) (locus MIRU 26). Locus VNTR 1982 is part of the Rv1753c (PPE PPE (Brit) n abbr (Univ) (= philosophy, politics, and economics) → Studiengang bestehend aus Philosophie, Politologie und Volkswirtschaft PPE n abbr (BRIT ) (SCOL 24), which belongs to the group of genes encoding PPE proteins and which has been argued to be responsible for antigenic variation Antigenic variation is the process by which an infectious organism alters its surface proteins in order to evade a host immune response. This change in antigenic profile may occur as the pathogen passes through a host population (also called "antigenic diversity") or may take place of M. tuberculosis (37). In our study, the degree of polymorphism at this locus was considerably higher than that previously reported for a panel of M. bovis isolates (27). By contrast, loci 2163a, 1955, 3336, and 3690, which were reported to be polymorphic for M. bovis, demonstrated low polymorphism in our study of M. tuberculosis Beijing isolates. We speculate that the presence of variation at a small number of loci in genes likely to be involved in the earliest interactions of pathogen Pathogen Any agent capable of causing disease. The term pathogen is usually restricted to living agents, which include viruses, rickettsia, bacteria, fungi, yeasts, protozoa, helminths, and certain insect larval stages. and host against a background of homogeneity at other loci suggests that these regions may be involved in the successful transmission of Beijing family strains. For the whole population studied, a small group of loci (VNTR 1982, VNTR 3232, MIRU 10, MIRU 26, MIRU 31, MIRU 39, MIRU 40, and ETR-A) offered the most discriminating panel and may be considered an essential part of the prospective universal panel of VNTR loci suitable for differentiation of M. tuberculosis isolates in different geographic settings with variable prevalence of highly conserved genotypes. The application of a limited number of loci (MIRU 10, MIRU 26, MIRU 31, VNTR 3232, and VNTR 1982) independently or in combination with other loci, may be a useful and rapid tool for differentiating strains within the Beijing family and for practical prospective genotyping and tracing of TB outbreaks in populations where the Beijing genotype predominates. Given the limited number of loci, analyzing this panel with a manual or automated approach is practical. In conclusion, our study shows that by expanding the VNTR panel beyond the 15-MIRU-ETR loci described previously, discrimination can be substantially increased. This method may be used for typing M. tuberculosis isolates, even for populations in which a particular genetic group is dominant. Acknowledgments We thank the bacteriologists at the Samara Oblast TB Reference Laboratory and Samara Oblast Health authorities and TB service for their help in sample collection, processing, and organizational issues, and staff of the UK Health Protection Agency (HPA (1) (High Performance Addressing) Refers to a variety of earlier addressing techniques that improved the quality of a passive matrix (LCD) screen. (2) (High Power A ) Mycobacterium mycobacterium Any of the rod-shaped bacteria that make up the genus Mycobacterium. The two most important species cause tuberculosis and leprosy in humans; another species causes tuberculosis in both cattle and humans. Reference Unit for their essential assistance and support. This study was funded by UK Department for International Development (CNTR CNTR Center CNTR Container CNTR Control CNTR Counter 000634) and a Foreign and Commonwealth Office Chevening Fellowship to V.N. (UKE0100129). References (1.) Raviglione MC. 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": the colliding epidemics of tuberculosis and HIV in Russia. Int J STD (Subscriber Trunk Dialing) Long distance dialing outside of the U.S. that does not require operator intervention. STD prefix codes are required and billing is based on call units, which are a fixed amount of money in the currency of that country. AIDS. 2004;15:641-6. (7.) Drobniewski F, Balabanova Y, Ruddy rud·dy adj. rud·di·er, rud·di·est 1. a. Having a healthy, reddish color. b. Reddish; rosy. 2. M, Weldon L, Jeltkova K, Brown T, et al. Rifampin- and Multidrug-resistant tuberculosis in Russian civilians and prison inmates: dominance of the Beijing strain family. Emerg Infect Dis. 2002;8:1320-6. (8.) Toungoussova OS, Sandven P, Mariandyshev AO, Nizovtseva NI, Bjune G, Cougant DA. Spread of drug-resistant Mycobacterium tuberculosis strains of the Beijing genotype in the Archangel archangel, in religion archangel (ärk`ānjəl), chief angel. They are four to seven in number. Sometimes specific functions are ascribed to them. The four best known in Christian tradition are Michael, Gabriel, Raphael, and Uriel. oblast oblast (ō`bläst, ŏ`–, Rus. ô`bləstyə) [Rus.,=region], administrative and territorial division in Russia, Ukraine, Belarus, and the former USSR. , Russia. J Clin Microbiol. 2002;40:1930-7. (9.) van Soolingen D. Molecular epidemiology molecular epidemiology Molecular medicine An evolving field that combines the tools of standard epidemiology–case studies, questionnaires and monitoring of exposure to external factors with the tools of molecular biology–eg, restriction endonucleases, of tuberculosis and other mycobacterial infections: main methodologies and achievements. J Intern intern /in·tern/ (in´tern) a medical graduate serving in a hospital preparatory to being licensed to practice medicine. in·tern or in·terne n. Med. 2001;249:1-26. (10.) Braden CR, Crawford JT, Schable BA. Assessment of Mycobacterium tuberculosis genotyping in a large laboratory network. Emerg Infect Dis. 2002;8:1210-5. (11.) McHugh TD, Dickens A, Gillespie SH. False molecular clusters due to non-random association of IS6110 with Mycobacterium tuberculosis. J Clin Microbiol. 2000;38:2081-6. (12.) Kanduma E, McHugh TD, Gillespie SH. Molecular methods for Mycobacterium tuberculosis strain typing: a users guide. J Appl Microbiol. 2003;94:781-91. (13.) Glynn JR, Whiteley J, Bifani PJ, Kremer K, van Soolingen D. Worldwide occurrence of Beijing/W strains of Mycobacterium tuberculosis: a systematic review. Emerg Infect Dis. 2002;8:843-9. (14.) Kremer K, Glynn JR, Lillebaek T, Niemann S, Kurepina N, Kreiswirth B, et ah Definition of the Beijing/W Lineage of Mycobacterium tuberculosis on the Basis of Genetic Markers. J Clin Microbiol. 2004;42:4040-9. (15.) Milan SJ, Hauge K, Kurepina N, Lofy K, Goldberg S, Narita M, et al. Expanded geographical distribution the natural arrangements of animals and plants in particular regions or districts. See under Distribution. See also: Distribution Geographic of the N family of Mycobacterium tuberculosis strain within the United States. J Clin Microbiol. 2004;42:1064-8. (16.) Sreevatsan S, Pan X, Stockbauer K, Connell N, Kreiswirth B, Whittam T, et al. Restricted structural gene polymorphism in the Mycobacterium tuberculosis complex indicates evolutionarily recent global transmission. Proc Natl Acad Sci U S A. 1997;94:9869-74. (17.) Plikaytis BB, Marden J, Crawford J, Woodley C, Buter W, Shinnik T. Multiplex PCR assay specific for the multidrug-resistant strains W of Mycobacterium tuberculosis. J Clin Microbiol. 1994;32:1542-6. (18.) Drobniewski F, Balabanova Y, Nikolayevskyy V, Ruddy M, Kuznetzov S, Zakharova S, et al. Drug-resistant TB, clinical virulence, and the dominance of the Beijing strain family in Russia. JAMA JAMA abbr. Journal of the American Medical Association . 2005;293:2726-31. (19.) Frothingham R, Meeker-O'Connell WA. Genetic diversity in the Mycobacterium tuberculosis complex based on variable numbers of tandem repeats. Microbiology. 1998;144:1189 96. (20.) Cowan LS, Mosher A mosher is a person who is crossed between goth/punk/skater they have long hair and listen to music like slipknot and metal music. Some people call them headbangers. At certain music shows they have something called a mosh pit, basically its a fight pit with loads of people bashing each other. L, Diem L, Massey JP, Crawford JT. Variable-number tandem repeats typing of Mycobacterium tuberculosis isolates with low copy numbers of IS6110 by using mycobacterial interspersed repetitive units. J Clin Microbiol. 2002;40:1592-602. (21.) Supply P, Mazars E, Lesjean S, Vincent V, Gicquel B, Locht C. Variable human minisatellite-like regions in the Mycobacterium tuberculosis" genome. Mol Microbiol. 2000;36:762-71. (22.) Supply P, Lesjean S, Savine E, Kremer K, van Soolingen D, Locht C. Automated high-throughput genotyping for study of global epidemiology of Mycobacterium tuberculosis based on mycobacterial interspersed repetitive units. J Clin Microbiol. 2001;39:3563-71. (23.) Sola C, Filliol I, Legrand E, Lesjean S, Locht C, Supply P, et al. Genotyping of the Mycobacterium tuberculosis complex using MIRUs: association with VNTR and spoligotyping for molecular epidemiology and evolutionary genetics Evolutionary genetics is the broad field of studies that attempts to account for evolution in terms of changes in gene and genotype frequencies within populations and the processes that convert the variation with populations into more or less permanent variation between species. . Infect Genet genet: see civet. Evoh 2003;3: 125-33. (24.) Roring S, Scott A, Brittain D, Walker l, Hewinson RG, Neill S, et ah Development of variable-number tandem repeat typing of Mycobacterium bovis Mycobacterium bovis A mycobacterium that causes a TB-like infection in cows; before pasteurization was common, M bovis spread to humans via contaminated milk : comparison of results with those obtained by using existing exact tandem repeats and spoligotyping. J Clin Microbiol. 2002;40:2126-33. (25.) Roring S, Scott AN, Hewinson RG, Neill SD, Skuce RA. Evaluation of variable number tandem repeat (VNTR) loci in molecular typing of Mycobacterium bovis isolates from Ireland. Vet Microbiol. 2004; 101:65-73. (26.) Le Fleche flèche n. A slender spire, especially one on a church above the intersection of the nave and transepts. [French, arrow, flèche, from Old French, arrow, of Germanic origin; see P, Fabre M, Denoeud F, Koeck J-L, Vergnaud G. High resolution, on-line identification of strains from the Mycobacterium tuberculosis complex based on tandem repeat typing. BMC (BMC Software, Inc., Houston, TX, www.bmc.com) A leading supplier of software that supports and improves the availability, performance, and recovery of applications in complex computing environments. Microbiol 2002;2:37-48. (27.) Skuce RA, MeCorry TP, McCarroll JF, Roring SM, Scott AN, Brittain D, et ah Discrimination of Mycobacterium tuberculosis complex bacteria using novel VNTR-PCR targets. Microbiology. 2002;148: 519-28. (28.) Ruddy M, Balabanova Y, Graham C, Fedorin I, Malomanova N, Elisarova E, et al. Rates of drug resistance and risk factor analysis in civilian and prison patients with tuberculosis in Samara Region, Russia. Thorax thorax, body division found in certain animals. In humans and other mammals it lies between the neck and abdomen and is also called the chest. The skeletal frame of the thorax is formed by the sternum (breastbone) and ribs in front and the dorsal vertebrae in back. . 2005;60:130-5. (29.) Yates MD, Drobniewski FA, Wilson SM. Evaluation of a rapid PCR-based epidemiological typing method for routine studies of Mycobacterium tuberculosis. J Clin Microbiol 2002;40:712-4. (30.) Kamerbeek J, Schouls L, Kolk A, van Agterveld M, van Soolingen D, Kuijper S, et ah Simultaneous detection and strain differentiation of Mycobacterium tuberculosis for diagnosis and epidemiology. J Clin Microbiol. 1997;35:907-14. (31.) Hunter PR, Gaston MA. Numerical index of the discriminatory ability of typing systems: an application of Simpson's index of diversity. J Clin Microbiol. 1988;26:2465-6. (32.) Bifani P, Mathema B, Campo M, Moghazeh S, Nivin B, Shashkina E, et al. Molecular identification of streptomycin streptomycin (strĕp'tōmī`sĭn), antibiotic produced by soil bacteria of the genus Streptomyces and active against both gram-positive and gram-negative bacteria (see Gram's stain), including species resistant to other monoresistant Mycobacterium tuberculosis related to multidrug resistant W strain. Emerg Infect Dis. 2001;7: 842-8. (33.) Mokrousov I, Narvskaya O, Limeschenko E, Otten T, Vyshnevskiy B. Novel IS6110 insertion sites in the direct repeat locus of Mycobacterium tuberculosis' clinical strains from the St. Petersburg area of Russia and evolutionary and epidemiological considerations. J Clin Microbiol. 2002;40:1504-7. PMID PMID PubMed-Indexed for MEDLINE PMID Portable Multispectral Imaging Device PMID Process Management Improvement & Deployment PMID Physical Media Id PMID Performance Metric Identifier : 11923382 (34.) Mokrousov I, Narvskaya O, Limeschenko E, Vyazovaya A, Otten T, Vyshnevskiy B. Analysis of the allelic diversity of the mycobacterial interspersed repetitive units in Mycobacterium tuberculosis strains of the Beijing family: practical implications and evolutionary considerations. J Clin Microbiol 2004;42:2438-44. (35.) Hawkey PM, Smith EG, Evans JT, Monk P, Bryan G, Mohamed HH, et al. Mycobacterial interspersed repetitive unit typing of Mycobacterium tuberculosis compared to IS6110-based restriction fragment length polymorphism analysis for the investigation of apparently clustered cases of tuberculosis. J Clin Microbiol. 2003;41:3514-20. (36.) Sun Y-J, Bellamy R, Lee AS, Ng ST, Ravindran S, Wong S-Y, et al. Use of mycobacterial interspersed repetitive unit-variable-number tandem repeat typing to examine genetic diversity of Mycobacterium tuberculosis in Singapore. J Clin Microbiol. 2004;42:1986-93. (37.) Cole ST, Brosch R, Parkhill J. 39 other authors. Deciphering the biology of Mycobacterium tuberculosis from the complete genome sequence. Nature. 1998;393:537-44. Vladyslav Nikolayevskyy, * Krishna Gopaul, * Yanina Balabanova, * ([dagger]) Timothy Brown Timothy Brown or Tim Brown may refer to:
* Barts and the London School of Medicine, University of London For most practical purposes, ranging from admission of students to negotiating funding from the government, the 19 constituent colleges are treated as individual universities. Within the university federation they are known as Recognised Bodies , London, United Kingdom; and ([dagger]) Samara Regional Tuberculosis Service, Samara, Russia Dr Nikolayevskyy is a postdoctoral post·doc·tor·al also post·doc·tor·ate adj. Of, relating to, or engaged in academic study beyond the level of a doctoral degree. Noun 1. research assistant at the HPA Mycobacterium Reference Unit, Institute of Cell and Molecular Sciences, Barts and The London School of Medicine, University of London. His research interests include different aspects of the clinical microbiology Clinical microbiology The adaptation of microbiological techniques to the study of the etiological agents of infectious disease. Clinical microbiologists determine the nature of infectious disease and test the ability of various antibiotics to inhibit or kill , epidemiology, and molecular genetics molecular genetics n. The branch of genetics that deals with hereditary transmission and variation on the molecular level. of M. tuberculosis. Address for correspondence: Francis Drobniewski, HPA Mycobacterium Reference Unit, Institute of Cell and Molecular Science, Barts and The London School of Medicine, University of London, 2 Newark St, E1 2AT, London, UK; email: f.drobniewski@qmul.ac.uk
Table 1. Baseline clinical and sociodemographic parameters of
187 tuberculosis (TB) patients
Isolates from Isolates from
civilian patients prisoners
Parameters (N = 138), n (%) (N = 49), n (%)
Mean age, y (SD) 42.4 (14.3) 32.5 (10.6)
Sex
Male 117 (84.8) 49 (100.0)
Female 21 (15.2) 0
TB treatment
New cases 105 (76.1) 36 (73.5)
Previously treated 33 (23.9) 13 (26.5)
HIV infected 4 (2.9) 5 (10.2)
Extensive lesions 35 (25.4) 12 (24.5)
shown on radiograph
Contact with TB patient 54 (39.1) 25 (51.0)
Selected sociologic
parameters
Smoker 103 (74.6) 46 (93.9)
Alcohol consumption 121 (87.7) 39 (79.6)
Drug use 9 (6.5) 20 (40.8)
Table 2. Prevalence of Beijing strains in clusters (15-loci
MIRU-ETR analysis) * ([dagger])
No. repeats in MIRU-ETR loci
MIRU
Cluster no. Size 2 4 10 16 20 23 24
1 3 2 2 3 1 2 5 1
2 2 2 2 3 3 2 6 1
3 3 2 2 3 3 2 5 1
4 75 2 2 3 3 2 5 1
5 3 2 3 3 3 2 5 1
6 2 2 2 1 3 2 5 1
7 31 2 2 3 3 2 5 1
8 2 2 2 3 3 2 5 1
9 2 2 2 7 2 2 5 1
10 3 1 2 4 3 2 5 1
No. repeats in MIRU-ETR loci
MIRU ETR
Cluster no. 26 27 31 39 40 A B C
1 4 3 3 2 4 3 2 3
2 5 3 3 2 5 3 2 3
3 5 3 4 3 3 4 2 3
4 5 3 5 3 3 4 2 3
5 5 3 5 3 3 4 2 3
6 7 3 5 3 3 4 2 3
7 7 3 5 3 3 4 2 3
8 3 3 6 3 3 4 2 3
9 1 3 2 2 3 4 2 4
10 5 3 2 2 5 2 2 1
* MIRU, Mycobacterial interspersed repetitive units, ETR, exact
tandem repeats.
([dagger]) Clusters 3-8 had 100% Beijing strains; the other
clusters had none.
Table 3. Frequency of occurrence of MIRU-ETR alleles and allelic
diversity at each locus for all strains *
No. repeats
Locus 0 1 2 3 4 5 6 7 8 9
MIRU 2 0 11 172 3 0 0 1 0 0 0
MIRU 4 0 2 182 3 0 0 0 0 0 0
MIRU 10 0 2 3 166 15 3 1 5 1 1
MIRU 16 0 24 7 156 0 0 0 0 0 0
MIRU 20 0 1 186 1 0 0 0 0 0 0
MIRU 23 0 2 0 0 0 173 9 3 0 0
MIRU 24 0 187 0 0 0 0 0 0 0 0
MIRU 26 0 7 0 2 11 122 5 40 0 0
MIRU 27 1 0 2 184 0 0 0 0 0 0
MIRU 31 0 1 20 31 7 124 4 0 0 0
MIRU 39 0 0 52 135 0 0 0 0 0 0
MIRU 40 2 3 7 147 14 13 1 0 0 0
ETR-A 0 3 18 28 138 0 0 0 0 0
ETR-B 0 0 187 0 0 0 0 0 0 0
ETR-C 0 11 9 157 10 0 0 0 0 0
No.
Locus HGDI AV
MIRU 2 0.151 4
MIRU 4 0.053 3
MIRU 10 0.206 9
MIRU 16 0.288 3
MIRU 20 0.011 3
MIRU 23 0.142 4
MIRU 24 0 1
MIRU 26 0.526# ([dagger]) 6
MIRU 27 0.032 3
MIRU 31 0.622# 6
MIRU 39 0.404# 2
MIRU 40 0.372# 7
ETR-A 0.426# 4
ETR-B 0 1
ETR-C 0.288 4
* N = 187; MIRU, mycobacterial interspersed repetitive units; ETR,
exact tandem repeats, HGDI, Hunter-Gaston diversity index, AV,
allelic variants.
([dagger]) Boldface loci showed at least moderate discriminative
power as defined by Sola et al. (23) and were the most promising
loci. Other loci provided poor discrimination or were monomorphic.
Note: Boldface loci showed at least moderate discriminative power
as defined by Sola et al indicated with #.
Table 4. Frequency of MIRU-ETR alleles and allelic diversity at each
locus for Beijing strains only *
No. repeats
Locus 0 1 2 3 4 5 6 7 8 9
MIRU 2 0 0 127 1 0 0 1 0 0 0
MIRU 4 0 0 126 3 0 0 0 0 0 0
MIRU 10 0 2 1 126 0 0 0 0 0 0
MIRU 16 0 1 0 128 0 0 0 0 0 0
MIRU 20 0 0 129 0 0 0 0 0 0 0
MIRU 23 0 0 0 0 0 128 0 1 0 0
MIRU 24 0 129 0 0 0 0 0 0 0 0
MIRU 26 0 0 0 2 1 89 0 37 0 0
MIRU 27 0 0 0 129 0 0 0 0 0 0
MIRU 31 0 1 0 1 6 117 4 0 0 0
MIRU 39 0 0 1 128 0 0 0 0 0 0
MIRU 40 0 0 1 127 0 1 0 0 0 0
ETR-A 0 0 0 3 126 0 0 0 0 0
ETR-B 0 0 129 0 0 0 0 0 0 0
ETR-C 0 1 0 128 0 0 0 0 0 0
No.
Locus HGDI AV
MIRU 2 0.031 3
MIRU 4 0.046 2
MIRU 10 0.046 3
MIRU 16 0.016 2
MIRU 20 0 1
MIRU 23 0.016 2
MIRU 24 0 1
MIRU 26 0.446# ([dagger]) 4
MIRU 27 0 1
MIRU 31 0.176# ([dagger]) 5
MIRU 39 0.016 2
MIRU 40 0.031 3
ETR-A 0.046 2
ETR-B 0 1
ETR-C 0.016 2
* N = 129; MIRU, mycobacterial interspersed repetitive units; ETR,
exact tandem repeats; HGDI, Hunter-Gaston diversity index; AV,
allelic variants.
([dagger]) Boldface loci showed at least moderate discriminative
power as defined by Sola et al. (23) and were the most promising
loci. Other loci provided poor discrimination or were monomorphic.
Note: Boldface loci showed at least moderate discriminative power
as defined by Sola et al. (23) and were the most promising loci.
Table 5. Frequency of an expanded set of 25 VNTR-MIRU alleles and
allelic diversity for each locus for Beijing strains * ([dagger])
No. repeats
Locus 1 2 3 4 5 6 7 8 9 10 12
424 0 1 3 125 0 0 0 0 0 0 0
531 0 0 0 0 0 0 0 0 0 0 0
1955 1 4 1 122 1 0 0 0 0 0 0
1982 0 1 0 1 3 34 2 86 2 0 0
2074 0 129 0 0 0 0 0 0 0 0 0
2163a 0 1 0 0 2 5 0 1 117 1 2
3232 0 0 1 0 0 0 0 0 1 3 62
3239 0 2 126 0 1 0 0 0 0 0 0
3336 0 1 0 0 1 0 124 2 1 0 0
3690 1 128 0 0 0 0 0 0 0 0 0
No. repeats
No.
Locus 13 14 15 16 17 20 25 26 HGDI AV
424 0 0 0 0 0 0 0 0 0.061 3
531 0 0 0 0 0 0 128 1 0.016 2
1955 0 0 0 0 0 0 0 0 0.105 4
1982 0 0 0 0 0 0 0 0 0.489 7
2074 0 0 0 0 0 0 0 0 0 1
2163a 0 0 0 0 0 0 0 0 0.177 7
3232 1 50 5 3 1 2 0 0 0.621 10
3239 0 0 0 0 0 0 0 0 0.046 3
3336 0 0 0 0 0 0 0 0 0.076 5
3690 0 0 0 0 0 0 0 0 0.016 2
* N = 129, VNTR, variable-number tandem repeats; MIRU, mycobacterial
interspersed repetitive units, HGDI, Hunter-Gaston discriminatory
index; AV, allelic variants.
([dagger]) No loci had allelic variants with 11, 18, 19, and 21-24
repeats.
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