Mycobacterium africanum cases, California.Five Mycobacterium tuberculosis Mycobacterium tuberculosis n. Tubercic bacillus. Mycobacterium tuberculosis complex isolates in California were identified as M. africanum by spoligotyping, single nucleotide polymorphisms, a deletion mutation, and phenotypic traits, confirming it as a cause of tuberculosis 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. . Three of the five patients from whom M. africanum was isolated had lived in Africa. ********** Mycobacterium africanum Mycobacterium africanum Epidemiology M.africanum is most commonly found in West African countries, causing up to a quarter of cases of tuberculosis in countries such as the Gambia. is a member of the 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. complex, which has been isolated from humans in equatorial Africa Equatorial Africa is an ambiguous term that is sometimes used to refer to tropical Africa, Sub-Saharan Africa, or the region of Africa traversed by the equator. The term is often used in tropical medicine and climatological discourse, but during colonial times it had a more . The disease produced by M. africanum is similar to that caused by M. tuberculosis or bovis, and like M. tuberculosis, this organism is likely spread by aerosol transmission (1). Human tuberculosis caused by M. africanum has been reported in Europe (2,3). However, we are unaware of previous reports of disease caused by M. africanum in the United States. The Study M. africanum may be identified by spoligotyping (4), by specific deletion mutations (5), DNA fingerprinting DNA fingerprinting or DNA profiling, any of several similar techniques for analyzing and comparing DNA from separate sources, used especially in law enforcement to identify suspects from hair, blood, semen, or other biological materials found at by IS6110 restriction fragment length polymorphisms 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 (RFLP RFLP abbr. restriction fragment length polymorphism RFLP restriction fragment length polymorphism. RFLP ) (4), or a combination of these methods. Isolates were initially identified as M. tuberculosis complex by using the AccuProbe system (Gen-Probe; San Diego San Diego (săn dēā`gō), city (1990 pop. 1,110,549), seat of San Diego co., S Calif., on San Diego Bay; inc. 1850. San Diego includes the unincorporated communities of La Jolla and Spring Valley. Coronado is across the bay. , CA). The isolates then underwent IS6110-based RFLP fingerprinting. The RFLP analyses were performed 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. the method of van Embden et al. (6). In addition to providing genotyping results, RFLP fingerprinting confirmed the identification obtained with Accuprobe. All strain typing was performed in-house at the Microbial microbial pertaining to or emanating from a microbe. microbial digestion the breakdown of organic material, especially feedstuffs, by microbial organisms. Diseases Laboratory, California Department of Health Services Department of Health Services may refer to:
The San Francisco Bay Area, colloquially known as the Bay Area or The Bay . Three isolates (from patients A, B, and C) were initially suspected of being M. africanum because of an epidemiologic association with Africa. These isolates were fingerprinted by IS6110 RFLP and by spoligotyping (8). All three were found to have the "signature" spoligotype described by Viana-Niero et al. as being characteristic of M. africanum (4), namely, they were missing spacers 8, 9, and 39 but had spacers 40-43. Using BioImage software, we searched the laboratory's database fur IS6110 fingerprints that matched those of the three cases with an African connection. This search yielded an additional two matches, cases D and E. Isolates from cases D and E were then genotyped by using spoligotyping and found to have the M. africanum signature spoligotype. The five M. africanum isolates were further characterized by performing standard biochemical identification tests and testing for susceptibility to pyrazinamide (PZA PZA Pyrazinamide, see there ). Niacin niacin: see coenzyme; vitamin. niacin or nicotinic acid or vitamin B3 Water-soluble vitamin of the vitamin B complex, essential to growth and health in animals, including humans. production and nitrate reduction were detected as described by Kent and Kubica (9). Susceptibility to PZA was determined by using the BACTEC radiometrie assay performed according to the method of Salfinger et al. (10). The M. africanum isolates were then examined to determine whether they had the RD9 deletion and specific oxyR and katG sequence mutations. Brosch et al. had reported that isolates of M. tuberculosis do not have the RD9 deletion, whereas other members of the M. tuberculosis complex, including M. bovis, microti, and M. africanum have this deletion (5). Two sets of primers for detecting the RD9 deletion, designed as described by Brosch et al., were obtained from Alex Pym at Stanford University Stanford University, at Stanford, Calif.; coeducational; chartered 1885, opened 1891 as Leland Stanford Junior Univ. (still the legal name). The original campus was designed by Frederick Law Olmsted. David Starr Jordan was its first president. . A [approximately equal to] 480-bp region was amplified by polymerase chain reaction polymerase chain reaction (pŏl`ĭmərās') (PCR), laboratory process in which a particular DNA segment from a mixture of DNA chains is rapidly replicated, producing a large, readily analyzed sample of a piece of DNA; the process is (PCR PCR polymerase chain reaction. PCR abbr. polymerase chain reaction Polymerase chain reaction (PCR) ) from M. africanum by using the flanking primers, and a [approximately equal to] 375-bp region was amplified from M. tuberculosis by using the internal primers. After an initial denaturation denaturation, term used to describe the loss of native, higher-order structure of protein molecules in solution. Most globular proteins exhibit complicated three-dimensional folding described as secondary, tertiary, and quarternary structures. step of 10 min at 95[degrees]C, amplification was performed for 35 cycles at 95[degrees]C for 30 s, 55[degrees]C for 1 min, and 72[degrees]C for 4 min, and a final step of elongation at 72[degrees]C for 10 min. The final concentration of each component in the 50-[micro]L PCR reaction tube was 1x PCR buffer, 2.5 mmol/L of Mg[Cl.sub.2], and 1.5 U of AmpliTaq Gold polymerase using AmpliTaq Gold kit with GeneAmp 10x PCR buffer II and Mg[Cl.sub.2] solution (Applied Biosystems Applied Biosystems, Inc. (formerly NASDAQ: ABIO) is the original name of a pioneer biotechnology company founded in 1981 in Foster City, California, among the Silicon Valley cities of the southern San Francisco Bay Area. , Foster City, CA), 1.25 mmol/L of deoxynucleotide triphosphate triphosphate /tri·phos·phate/ (tri-fos´fat) a salt containing three phosphate radicals. tri·phos·phate n. A salt or ester containing three phosphate groups. mix (Applied Biosystems), 0.2 [micro]mol/L of each primer, 5 [micro]L of 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. template. A M. tuberculosis strain, H37Rv, and M. africanum strain ATCC ATCC American Type Culture Collection, see there 25420 were included in PCR runs as reference strains. A 548-bp region of the oxyR locus was amplified by PCR using the primer sequences described by Sreevatsen et al. (11). After an initial denaturation step of 4 min at 95[degrees]C, amplification was performed for 30 cycles with the following parameters: 95[degrees]C for 30 s, 55[degrees]C for 30 s, and 72[degrees]C for 45 s. A final elongation step was performed for 5 min at 72[degrees]C. For katG, a primer set, 5'-TGCTGGCGCTTGGCAATACA and 5'-GCCGCGCTTGTCGCTACC, was designed to amplify a 429-bp region encompassing codon codon: see nucleic acid. 463. With the exception of an annealing annealing (ənēl`ĭng), process in which glass, metals, and other materials are treated to render them less brittle and more workable. temperature of 60[degrees]C, the amplification parameters for katG were identical to those described for oxyR. The amplified products were purified by using QIAquick spin columns (Qiagen Inc., Valencia, CA) and subjected to dRhodamine Terminator Cycle Sequencing (Applied Biosystems, Foster City, CA) as recommended by the manufacturer. The cycle sequencing reactions were analyzed on an ABI Abi (ā`bī) [short for Abijah], in the Bible, King Hezekiah's mother. (Application Binary Interface) A specification for a specific hardware platform combined with the operating system. 377 DNA sequencer A DNA sequencer is an instrument used to automate the DNA sequencing process. DNA sequencers have become more important due to large genomics projects and the need to increase productivity. , and the sequences aligned with those derived from M. tuberculosis strain H37Rv and M. africanum strain ATCC 25420. For case histories, see Table 1. The five isolates were identified as M. tuberculosis complex by a positive result with the Gen-Probe AccuProbe system and by the presence of IS6110 insertion sequences. When spoligotyping was performed on isolates from cases A through E, all were found to have the M. africanum signature spoligotype, as described by Viana-Niero et al. (4). The results of spoligotyping are shown in the Figure. [FIGURE OMITTED] The five isolates were M. africanum, based on several criteria shown in Table 2. Susceptibility of the strains to PZA, nitrate reduction, production of niacin, and the presence of guanosine guanosine /gua·no·sine/ (gwah´no-sen) a purine nucleoside, guanine linked to ribose; it is a component of RNA and its nucleotides are important in metabolism. Symbol G. at oxyR285 were incompatible with identification of the isolates as M. bovis. The RD9 deletion was shown for all five isolates and the M. africanum reference strain, ATCC 25420, by 1) the presence of a [approximately equal to] 480-bp band on the agarose agarose more highly purified form of agar with similar uses to agar and widely used in the separation of nucleic acid fragments. gel when the PCR was performed with the flanking primers and 2) the absence of a [approximately equal to] 375-bp band when the PCR was performed with the internal primers. The RD9 deletion was incompatible with identification of the isolates as M. tuberculosis, and CTG CTG Cartridge CTG Center for Technology in Government (SUNY, Albany, New York) CTG Center for Technology in Government CTG Computer Task Group (IT consulting company; Buffalo, NY, USA) at katG463 suggested that the isolates were not M. tuberculosis, since most isolates of this species have CGG CGG Compagnie Generale de Geophysique CGG Cytosine-Guanine-Guanine CGG Canadian Grenadier Guards (Canadian reserve military unit) CGG Cancer Genetics Group (Birmingham, UK) at this site (7). Conclusions David et al. (12) and Frothingham et al. (13) reported that some isolates of M. africanum are resistant to PZA and fail to accumulate niacin, distinguishing them from most strains of M. tuberculosis, while other isolates are susceptible to PZA and produce niacin. These five isolates of M. africanum were susceptible to PZA, and three out of the five tested positive for niacin production and nitrate reduction (the remaining two cultures had lost viability and were not available for this testing). This rendered the cultures phenotypically indistinguishable from M. tuberculosis (12-14). For each of the reported cases, the signature M. africanum spoligotype pattern described by Viana-Niero et al. (4) was supported by the single nucleotide polymorphisms characteristic of M. africanum and by the RD9 mutation that characterizes members of the tuberculosis complex other than M. tuberculosis. At present, the Microbial Diseases Laboratory plans to spoligotype all strains of M. tuberculosis complex. Clinical features and drug susceptibility were not distinctive for M. africanum isolates, nor were all associated with patients who came from Africa. No connection with a source case from Africa was found for patients D or E. However, since spoligotyping will be routine, noting the signature africanum spoligotype may be worthwhile. This spoligotype may indicate an increased chance that the patient may have acquired the M. tuberculosis complex infection in Africa or possibly from an African source case.
Table 1. Clinical characteristics of patients with Mycobacterium
africanum disease
Demographic Clinical
Patient characteristics Signs and symptoms characteristics
A 25-y-old black 3 months' produc- Large left upper
South African man tive cough, weight lobe infiltrate on
with recent travel loss, and low- chest radiograph
to West Africa grade fever
B 34-y-old black 2 months' cough, Right lower lobe
West African woman fever, night cavitation,
recently arrived in sweats, fatigue streaky infil-
U.S. with metasta- trates bilaterally
tic carcinoma, on chest radio-
treated with chemo- graph, normocytic
therapy 1 year anemia
before presen-
tation.
C 26-y-old black Unknown Cavitary lesion on
South African, chest radiograph
immigrated to U.S.
2 y before diagno-
sis
D 26-y-old Vietnamese 2 weeks' produc- Unknown
man, immigrated to tive cough,
U.S. 6 y before positive PPD
diagnosis. No his-
tory of travel to
Africa or African
contacts with
tuberculosis
E 27-y-old U.S.-born 2 months' anorexia Normal chest
black man with no and weight loss; 1 radiograph re-
known risk factors month of cough and sults. Pancreatic
for tuberculosis night sweats; 1 cyst and fullness
infection. No week of fever and of left psoas
history of travel abdominal pain muscle on CT scan
to Africa or
African contacts
with tuberculosis
Patient Treatment (a) Outcome
A INH, rifampin, PZA, and Resolution of symptoms
ethambutol by directly and improvement of chest
observed therapy for 6 radiograph
months
B INH, rifampin, PZA, and Sputum culture negative
ethambutol by DOT after 2 weeks of therapy.
Only modest
improvement in chest
radiograph. Returned to
West Africa after 4
months DOT
C INH, rifampin, PZA, and Sputum culture and smear
ethambutol by DOT for 6 negative, chest
months radiograph improved
D Capreomycin, ofloxacin, Sputum smear and culture
PAS, clofazamine, and converted to negative,
cycloserine for 2 y by symptoms resolved. Free
DOT of disease 2 y after
therapy completed
E INH, rifampin, PZA, and Symptoms resolved. Free
ethambutol for 10 months of disease 1 y after
by DOT therapy completed
(a) INH, izoniazid; PZA, pyrazinamide; DOT. directly observed
therapy; CT, computerized tomography, PPD, purified protein
derivative; PAS, para-aminosalicylic acid.
Table 2. Phenotypic and molecular characteristics of Mycobacterium
africanum isolates and country of birth for five patients
No. of
copies of Spoligo-typing Codon
IS6110 pattern missing OxyR katG463
Patient (bands) spacers 8,9,39? 285 (a) sequence (b)
A 10 Yes G CTG
B 3 Yes G CTG
C 9 (f) Yes G CTG
D 11 Yes G CTG
E 9 Yes G CTG
Presence of
RD9 PZA Suscep- Niacin Nitrate
Patient deletion? tibility (c) production reduction (d)
A Yes S + 3+
B Yes S ND (e) ND
C Yes S ND ND
D Yes S + 4+
E Yes S + 3+
Major site
Patient of disease Birth country
A Lung South Africa
B Lung Ivory Coast
C Lung South Africa
D Lung Vietnam
E Pancreas USA
(a) Isolates of M. bovis do not have G to this site.
(b) CTG is found in M bovis and M. africanum, but not
in most strains of M. tuberculosis.
(c) S, susceptible; PZA, pyrazinamide.
(d) 3+ and 4+ reactions are considered positive.
(e) ND, not done (because the culture lost viability).
(f) Restriction fragment length polymorphism patterns
for isolates from patients C and E were identical.
References (1.) Adler JJ, Rose DN. Transmission and pathogenesis of tuberculosis. In: Rom WN, Garay SM, editors. Tuberculosis. Boston: Little, Brown, and Co.; 1996. p. 129-40. (2.) Grange JM, Yates MD. Incidence and nature of human tuberculosis due to Mycobacterium africanum in southeast England. Epidemiol Infect 1989;103:127-32. (3.) Grosset J, Decroix G, Sors C. Tuberculosis due to Mycobacterium africanum in African Negroes in the Paris area. Revue de Tuberculose et de Pneumologie (Paris) 1971;35:430 6. (4.) Viana-Niero C, Gutierrez C, Sola C, Filliol I, Boulahbal F, Vincent V, et al Genetic diversity of Mycobacterium africanum clinical isolates based on IS6110-restriction fragment length 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. analysis, spoligotyping, and variable number of tandem repeats. J Clin Microbiol 2001;39:57-5. (5.) Brosch R, Gordon SV, Marmiesse M, Brodin P, Buchrieser C, Eiglmeier K, et al. A new evolutionary scenario for the Mycobacterium tuberculosis complex. Proc Natl Acad Sci U S A 2002;99:3684-9. (6.) van Embden JDA JDA Japan Defense Agency JDA Joint Development Agreement JDA Janne da Arc (band) JDA Joint Duty Assignment JDA Jerusalem Development Authority JDA Jovian Detention Authority (gaming) , 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;31:40-9. (7.) Mazurek, GH, Cave MD, Eisenach KD, Wallace RJ, Bates Bates , Katherine Lee 1859-1929. American educator and writer best known for her poem "America the Beautiful," written in 1893 and revised in 1904 and 1911. JH, Crawford JT Chromosomal DNA fingerprint patterns produced with IS6110 as strain-specific markers for epidemiologic study epidemiologic study A study that compares 2 groups of people who are alike except for one factor, such as exposure to a chemical or the presence of a health effect; the investigators try to determine if any factor is associated with the health effect of tuberculosis. J Clin Microbiol 1991;29:2030-3. (8.) Kamerbeek J, Schouls L, Kolk A, van Agterveld M, van Soolingen D, Kuijper S, et al. Simultaneous detection and strain differentiation of Mycobacterium tuberculosis for diagnosis and epidemiology. J Clin Microbiol 1997;35:907 14. (9.) Kent P, Kubica G. Public health mycobacteriology: a guide for the level III laboratory. Atlanta: Centers for Disease Control; 1985. (10.) Salfinger M, Reller LB, Demchuk B, Johnson ZT. Rapid radiometric method for pyrazinamide susceptibility testing of Mycobacterium tuberculosis. Res Microbiol 1989;140:301-9. (11.) Sreevatsen S, Escalante E Pan X, Gillies DA II, Siddiqui S, Khalaf CN, et al. Identification of a polymorphic polymorphic - polymorphism nucleotide in oxyR specific for 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 . J Clin Microbiol 1996;34:2007-10. (12.) David HL, Jahan M-T, Jumin A, Grandry J, Lehman EH. Numerical taxonomy Numerical taxonomy The grouping by numerical methods of taxonomic units based on their character states. The application of numerical methods to taxonomy, dating back to the rise of biometrics in the late nineteenth century, has received a great deal of analysis of Mycobacterium africanum. Int J Syst Bacteriol 1978;28:467-72. (13.) Frothingham R, Strickland PL, Bretzel G, Ramaswamy S, Musser JM, Williams DL. Phenotypic and genotypic characterization of Mycobacterium africanum isolates from West Africa. J Clin Microbiol 1999;37:1921-5. (14.) Niemann S, Richter E, Rusch-Gerdes S. Differentiation among members of the Mycobacterium tuberculosis complex by molecular and biochemical features: evidence for two pyrazinamide-susceptible subtypes of M. bovis. J Clin Microbiol 2000;38:152-7. Dr. Desmond has worked at the Microbial Diseases Laboratory, California Department of Health Services, since 1990. His research interests include laboratory methods for detecting drug resistance in Mycobacterium tuberculosis and applications for molecular strain typing in the mycobacteriology laboratory. Address for correspondence: Edward Desmond, Microbial Diseases Laboratory, California Department of Health Services, 850 Marina Bay Parkway, Richmond, CA 93804, USA; fax: 510-412-3706; email: edesmond@dhs.ca.gov Edward Desmond, * Ameena T. Ahmed, * William S. Probert, * Janet Ely, * Yvonne Jang, * Cynthia A. Sanders, * Shou-Yean Lin, * and Jennifer Flood * * California Department of Health Services, Richmond, California, USA |
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