Rifampicin resistance in tuberculosis outbreak, London, England.Mycobacterium tuberculosis Mycobacterium tuberculosis n. Tubercic bacillus. Mycobacterium tuberculosis isolates cultured from 6 patients associated with an isoniazid-resistant M. tuberculosis outbreak acquired rifampicin rifampicin /rif·am·pi·cin/ (rif´am-pi-sin) rifampin. rifampin, rifampicin a derivative of rifamycin; an antibacterial and antifungal agent used in the treatment of mycobacterial infections, actinomycosis and histoplasmosis. resistance. The rpoB gene sequence showed that resistance was associated with rare mutations in each isolate. Three isolates had a mutation outside the rifampicin resistance-determining region. ********** In January 2000, 4 cases of smear-positive pulmonary tuberculosis (TB) caused by Mycobacterium tuberculosis in young men from the local community were identified during a 1-week period at a hospital in north London, United Kingdom (1). Three isolates were shown to be isoniazid-mono-resistant TB. Further investigation showed 155 confirmed or probable cases, 132 in London and 23 outside London, which suggests a large outbreak of a unique strain in the London area (2). Confirmed case-patients were defined as patients with isolates of M. tuberculosis resistant to isoniazid isoniazid (ī'sōnī`əzĭd), drug used to treat tuberculosis. Also known as isonicotinic acid hydrazide, isoniazid is the most effective antituberculosis drug currently available. that had the same band pattern on restriction length polymorphism typing (RFLP RFLP abbr. restriction fragment length polymorphism RFLP restriction fragment length polymorphism. RFLP ); these patients were residents of London at the time of their diagnosis, which had been made since January 1995 (2). Probable cases were defined as for confirmed cases except that isolates underwent rapid epidemiologic typing [RAPET] but are awaiting RFLP typing (2). RAPET is a rapid screening molecular typing method developed at the 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 (MRU MRU Maximum Receive Unit (PPP) MRU Most Recently Used (opposite of LRU) MRU Motion Reference Unit MRU Multi-campus Research Unit MRU Magnetic Resonance Urography MRU Media Robot Utility ) (3). In October 2002, the TB isolate from 1 patient associated with the outbreak had developed resistance to rifampicin. Initially, the isolate was tested with a commercial line probe rifampicin resistance determining hybridization hybridization /hy·brid·iza·tion/ (hi?brid-i-za´shun) 1. crossbreeding; the act or process of producing hybrids. 2. molecular hybridization 3. assay, Inno-LiPA (Innogenetics Belgium, Gent, Belgium). However, the line probe assay failed to identify rifampicin resistance in this isolate, and rifampicin resistance was only detected on phenotypic antimicrobial sensitivity testing at MRU. Subsequently, 5 additional rifampicin-resistant isolates from different patients associated with this outbreak were identified at MRU. The aim of this study was to determine the basis for the rifampicin resistance in these 6 isolates by sequencing the entire rpoB gene. Rifampicin resistance can occur as a result of mutations on the rpoB gene that encodes the [beta]-subunit of RNA polymerase (4). More than 95% of these mutations occur on an 81-bp fragment of the gene between bases 1276 and 1356 (432-458 in the rpoB gene of M. tuberculosis and codon codon: see nucleic acid. 507-534 in the Escherichia coli rpoB gene) (5,6). This region is known as the rifampicin resistance-determining region (RRDR RRDR Raw Radar Data Recorder ), or "hotspot," and is used as a target for direct sequencing and commercial line probe assays. The Study The isoniazid-monoresistant and multidrug-resistant tuberculosis (MDR-TB MDR-TB Multi-Drug Resistant Tuberculosis ) isolates were obtained from the patients' source hospital or MRU. All isolates were identified as belonging to the same strain of M. tuberculosis (RAPET or IS6110 typing), and all drug-susceptibility testing was carried out at MRU according to standard procedures. The wildtype control isolate used for these studies was M. tuberculosis, H37Rv (ATCC ATCC American Type Culture Collection, see there , 9360 National Collection of Type Culture, London, UK). Three isolates, 018, 483, and 915, were from patients in whom MDR-TB developed as a result of poor compliance with therapy, whereas isolates 604, T7, and 371 were from patients who contracted primary MDR-TB. 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. was prepared from the 6 isolates of M. tuberculosis by emulsifying 2 3 colonies in 400 [micro]L Tris-EDTA buffer and heating the suspension in a water bath for 40 min at 80[degrees]C. 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) ) was performed on the extracted DNA with 6 sets of primers designed to amplify 6 overlapping fragments of the rpoB gene from the 6 M. tuberculosis isolates (Table). Ten microliters of DNA was added to the PCR mix containing 81.4 [micro]L PCR-quality water, 10 [micro]L potassium chloride buffer (Bioline Ltd., London, UK), 0.4 [micro]L of each primer (100 retool) (Sigma-Genosys Ltd., Haverhill, UK), 3 [micro]L deoxynucleoside triphosphates (5 mmol), and 1 [micro]L Taq (Bioline). The amplification was performed on a Techgene thermal cycler (Techne, Princeton, NJ, USA). PCR products were separated by gel electrophoresis on a 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, and DNA bands were stained with ethidium bromide. Primers and excess nucleotides were removed from the amplified DNA with a PCR clean-up kit (Qiagen, Inc., Valencia, CA, USA). The amount of DNA in the cleaned-up product was quantified by comparing the intensity of the band to bands of known intensity in a HyperLadder marker (Bioline). Forward and reverse cycle sequencing reactions were performed with the Big Dye Terminator Cycle Sequencing Ready Reaction DNA sequencing kit (Applied Biosystems, Inc., Foster City, CA, USA). Briefly, 40 ng of cleaned-up DNA was added to 10.8 [micro]L PCR-quality water, 3 [micro]L buffer, 3.2 [micro]L of forward or reverse 1 mmol primer, and 1 [micro]L of cycle sequencing ready reaction mix. The labeled DNA was precipitated by adding 14.5 [micro]L PCR-quality water, 62.5 [micro]L 95% ethanol, and 3 [micro]L sodium acetate solution (2.3 mol/L) and centrifuging (13,000 x g, 15 min, 4[degrees]C). The supernatant supernatant /su·per·na·tant/ (-na´tant) the liquid lying above a layer of precipitated insoluble material. supernatant the liquid lying above a layer of precipitated insoluble material. was removed with a fine-tipped pipette pipette /pi·pette/ (pi-pet´) [Fr.] 1. a glass or transparent plastic tube used in measuring or transferring small quantities of liquid or gas. 2. to dispense by means of a pipette. , and the pellet was cleaned with 200 [micro]L 70% ethanol and then recentrifuged (13,000 x g, 15 min, 4[degrees]C). Again the supernatant was removed, and the pellet was dried at 37[degrees]C for 30 min. Four microliters of formamide and 1 [micro]L of dextran dextran /dex·tran/ (dek´stran) a high-molecular-weight polymer of d-glucose, produced by enzymes on the cell surface of certain lactic acid bacteria. loading buffer were added to each pellet, and 1.5 [micro]L of sample was added to each well of the sequencing gel. The 6 fragments of the rpoB gene from each of the 6 isolates were then sequenced with 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 Applied Biosystems 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. . The sequences obtained from each isolate were joined together to form a continuous whole gene sequence, aligned with ClustalW (http://www.ebi.ac. uk/clustalw/) and compared to the wildtype to identify base-pair mismatches. In addition, all 6 isolates were tested with a line probe resistance-determining hybridization assay, Inno-LiPA (Innogenetics Belgium), as described in the manufacturer's instructions. Briefly, an 81-bp region of the rpoB gene was amplified with biotinylated primers, which yielded a biotinylated target sequence, and hybridized with specific oligonucleotide probes immobilized on a parallel strip. After hybridization, streptavidin labeled with alkaline phosphatase was used to detect any hybrids, Inno-LiPA consists of 10 oligonucleotide probes (19-23 bases in length), encompassing the 81-bp region (RRDR) of the rpoB gene. One is specific for M. tuberculosis complex, whereas the other 5 partially overlapping wildtype probes (S1-S5) cover the region from positions 507 to 534 of the rpoB gene. These S-probes hybridize hy·brid·ize intr. & tr.v. hy·brid·ized, hy·brid·iz·ing, hy·brid·iz·es 1. To produce or cause to produce hybrids; crossbreed. 2. to the wildtype (rifampicin-sensitive) DNA sequence. Failure of any of these S-probes to hybridize indicates that a mutation has occurred. Four other probes (R2, R4a, R4b, and R5) are specific for amplicons carrying the most common rpoB mutation that confers rifampicin resistance. The results of the Inno-LiPA assay showed 5 of the 6 isolates, which were phenotypically rifampicin-resistant, were negative. The target DNA hybridized to all 5 wildtype S-probes and none of the R-probes, which demonstrated that the assay failed to detect rifampicin resistance in these 5 isolates. The Inno-LiPA assay cannot detect mutations outside the RRDR. Failure to detect rare mutations within the RRDR may be caused by nonspecific nonspecific /non·spe·cif·ic/ (non?spi-sif´ik) 1. not due to any single known cause. 2. not directed against a particular agent, but rather having a general effect. nonspecific 1. hybridization of the wildtype S-probes because of slight fluctuations in temperature during the hybridization process. Isolate 483 showed a weak DNA hybridization reaction with the S4 probe, indicating that a mutation was present on codon 451 (codon 526 in Escherichia coli). The exact nature of the mutation could not be determined with this assay. Analysis of the sequence data identified specific mutations in rpoB in all 6 strains studied (Figure 1). Three had mutations within the RRDR, and of these, 2 were C-to-G mutations at codon 456, inducing a serine serine (sĕr`ēn), organic compound, one of the 20 amino acids commonly found in animal proteins. Only the l-stereoisomer appears in mammalian protein. to tryptophan tryptophan (trĭp`təfăn), organic compound, one of the 20 amino acids commonly found in animal proteins. Only the l-stereoisomer appears in mammalian protein. amino acid conversion ($456W). The third was an A-to-G mutation at codon 451, resulting in a change from histidine histidine (hĭs`tĭdēn), organic compound, one of the 22 α-amino acids commonly found in animal proteins. Only the l-stereoisomer appears in mammalian protein. to arginine arginine (är`jənĭn), organic compound, one of the 20 amino acids commonly found in animal proteins. Only the l-stereoisomer participates in the biosynthesis of proteins. (H451R) (Figure 1). No other mutations were identified in the DNA sequences outside the RRDR in these 3 isolates. The 3 other isolates had the mutation G to T at codon 176, outside the RRDR, which caused a change from valine valine (văl`ēn), organic compound, one of the 22 α-amino acids commonly found in animal proteins. Only the l-stereoisomer appears in mammalian protein. to phenylalanine phenylalanine (fĕn'əlăl`ənēn'), organic compound, one of the 22 α-amino acids commonly found in animal proteins. Only the l-stereoisomer appears in mammalian protein. (V176F). Neither RRDR mutations nor any other mutations were/bund in the rpoB gene sequences of these 3 isolates. [FIGURE 1 OMITTED] Of the mutations found within the RRDR, H526R occurs in <4%, and S531W occurs in [approximately equal to] 1.4% of all rifampicin-resistant isolates, respectively (7). Mutations outside the RRDR account for <4% of rifampicin resistance, and few have been described (7-9). In a previous study (7), V176F was found in 5 of 18 isolates with no mutations in the RRDR from Asia (9,10) and Africa (11,12). To our knowledge, this is the first time this type of mutation has been detected in strains isolated in the United Kingdom. Three different mutations in the rpoB gene, V176F, H526R and S531W, were detected in the isolates associated with the isoniazid-resistant outbreak. Given that all the mutations found in this study are rare and that MDR-TB developed during treatment in 3 patients (018, 483, and 915) (Figure 2), the rifampicin-resistance mutations observed in these 3 patients likely occurred on 3 independent occasions, as a result of poor compliance with therapy. Two of these patients, 018 and 915, were contacts of the 3 patients who subsequently had primary MDR-TB (patients T7 and 604 [V176F] and 317 [S531W]) (Figure 2). [FIGURE 2 OMITTED] Conclusions Our study highlights problems associated with using a line probe hybridization assay to detect rifampicin resistance in M. tuberculosis. The Inno-LiPA assay cannot detect mutations outside the RRDR, and failure to detect rare mutations within the RRDR may be caused by nonspecific hybridization of the wildtype S-probes because of slight fluctuations in temperature during the hybridization process. In this study, all the rare mutations, inside and outside the RRDR, were detected by sequencing the entire rpoB gene. The inability to identify MDR-TB isolates results in treatment failure and increased risk for transmission of resistant disease in the community. We recommend that, when the index of suspicion index of suspicion Medtalk A phrase broadly used to indicate how seriously a particular disease is being entertained as a diagnosis; as an example, there is a high IOS that rapid and unexplained weight loss in an elderly Pt is due to pancreas CA, and a low IOS that for MDR-TB is high and the line probe assays fail to detect mutations conferring rifampicin resistance, the entire rpoB gene should be sequenced to prevent unnecessary delay in diagnosing MDR-TB.
Table. Sequences of 6 sets of primers designed to amplify
6 overlapping fragments of the rpoB gene from Mycobacterium
tuberculosis isolates
Fragment Amplicon size Primer position
1 697 by -135 to -112 *
541-562
2 688 by 451-472
1119-1139
3 706 by 1029-1048
1714-1735
4 681 by 1624-1645
2284-2305
5 811 by 2194-2215
2887-3005
6 847 by 2797-2815
+113 to +135 *
Fragment Primers
1 Forward 5' GTT TAG TTG CGT GCG TGC
Reverse 5' CTTGTCAAT GGT CTC GTC GAA
2 Forward 5' TTC CCG ATG ATG ACC GAG AAG
Reverse 5' GGA TCA GCT CGC CGA CCG TA
3 Forward 5' CGA GGG TCA GAC CAC GAT G
Reverse 5' GCG GGG CGA GAC GTC CAT GTA
4 Forward 5' ATC GAT GCG GAC GGT CGC TTC
Reverse 5' CGG GAT GTC GCG GGT GAT CTC
5 Forward 5' TCC AAC CGC CTG GTC GAA GAG
Reverse 5' CGT CGA CAC AAT GGC GTT
6 Forward 5' TGT GCC CAC AGC GGC TGG
Reverse 5' CTT TTT GAC CTC GCC ATA GGA C
* Denotes a primer position in the sequence before the start (-)
or after the end (+) of the rpoB gene sequence.
Acknowledgments We are grateful to Francis Drobniewski and Malcolm Yates for providing us with the MDR-TB isolates and to Sarah Batt and Clare Ling for their help with sequencing. References (1.) Ruddy MC, Davies AP, Yates MD, Yates S, Balasegaram S, Drabu Y, et al. Outbreak of isoniazid resistant tuberculosis in north London. 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. . 2004; 59:279-85. (2.) Davies AP, Ruddy MC, Neely F, Ruggles R, on behalf of the Outbreak Control Committee. Outbreak of isoniazid resistant tuberculosis in north London 1999-2004. Dulwich, London: Health Protection Agency Regional Epidemiology Unit; 2004. (3.) 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. (4.) Jin DJ, Gross CA. Mapping and sequencing of mutations in the Escherichia coli rpoB gene that lead to rifampicin resistance. J Mol Biol. 1988;202:45-58. (5.) Miller LP, Crawford JT, Shinnick TM. The rpoB gene of Mycobacterium tuberculosis. Antimicrob Agents Chemother. 1994;38:805-11. (6.) Ramaswamy S, Musser JM. Molecular genetic basis of antimicrobial agent resistance in Mycobacterium tuberculosis: 1998 update. Tuber tuber, enlarged tip of a rhizome (underground stem) that stores food. Although much modified in structure, the tuber contains all the usual stem parts—bark, wood, pith, nodes, and internodes. Lung Dis. 1998;79:3-29. (7.) Heep M, Brandstatter B, Rieger U, Lehn N, Richter E, Rusch-Gerdes S, et al. Frequency of rpoB mutations inside and outside the cluster I region in rifampin-resistant clinical Mycobacterium tuberculosis isolates. J Clio Microbiol. 2001;39:107-10. (8.) Kiepiela P, Bishop K, Kormuth E, Roux Roux , Pierre Paul Émile 1853-1933. French bacteriologist. His work with the diphtheria bacillus led to the development of antitoxins to neutralize pathogenic toxins. L, York DF. Comparison of PCR-heteroduplex characterization by automated DNA sequencing and line probe assay for the detection of rifampicin resistance in Mycobacterium tuberculosis isolates from KwaZulu-Natal, South Africa. Microb Drug Resist. 1998;4:263-9. (9.) Hirano K, Abe C, Takahashi M. Mutations in the rpoB gene of rifampin-resistant Mycobacterium tuberculosis strains isolated mostly in Asian countries and their rapid detection by line probe assay. J Clin Microbiol. 1999;37:2663-6. (10.) Yang B, Koga H, Ohno H, Ogawa K, Fukuda M, Hirakata Y, et al. Relationship between antimycobacterial activities of rifampicin, rifabutin and KRM-1648 and rpoB mutations of Mycobacterium tuberculosis. J Antimicrob Chemother. 1998;42:621-8. (11.) Caugant DA, Sandven P, Eng J, Jeque JT, Tonjum T. Detection of rifampin rifampin (rĭfăm`pĭn), antibiotic used in the treatment of tuberculosis. It is also used to eliminate the meningococcus microorganism from carriers and to treat leprosy, or Hansen's disease. resistance among isolates of Mycobacterium tuberculosis from Mozambique. Microb Drug Resist. 1995:1:321-6. (12.) Cockerill FR 3rd, Williams DE, Eisenach KD, Kline BC, Miller LK, Stockman L, et al. Prospective evaluation of the utility of molecular techniques for diagnosing nosocomial nosocomial /noso·co·mi·al/ (nos?o-ko´me-il) pertaining to or originating in a hospital. nos·o·co·mi·al adj. 1. Of or relating to a hospital. 2. transmission of multidrug-resistant tuberculosis. Mayo Clin Proc. 1996;71:221-9. Claire Jenkins, * Alleyna P. Claxton, ([dagger]) Robert J. Shorten, * Timothy D. McHugh, * and Stephen H. Gillespie * * Royal Free Hospital, London, United Kingdom; and ([dagger]) Homerton Hospital, London, United Kingdom Dr. Jenkins works as a registered clinical scientist in the Department of Microbiology at the Royal Free Hospital in London. Her research involves molecular typing and identification of pathogenic bacteria in general, with a specific interest in Mycobacterium species. Address for correspondence: Claire Jenkins, Department of Medical Microbiology, Royal Free Hospital, London, NW3 2QG, United Kingdom; tax: 44-20-7794-4433; email: claire.jenkins@royalfree.nhs.uk |
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