rpoB Gene mutations in rifampin-resistant Mycobacterium tuberculosis identified by polymerase chain reaction single-stranded conformational polymorphism. (Research).The use of polymerase chain reaction-single-stranded conformational 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. (PCR-SSCP PCR-SSCP Polymerase Chain Reaction–Single Strand Conformation Polymorphism ) to study rpoB gene mutations in rifampin-resistant (RIFr) Mycobacterium tuberculosis Mycobacterium tuberculosis n. Tubercic bacillus. Mycobacterium tuberculosis has yielded contradictory results. To determine the sensitivity of this method, we analyzed 35 RIFr strains and 11 rifampin-susceptible (RIFs) strains, using the DNA sequencing DNA sequencing The determination of the sequence of nucleotides in a sample of DNA. of the core region of rpoB for comparison. Of the RIFr, 24 had a PCR-SSCP pattern identical to that of H37Rv; the other 11 had four different patterns. The 11 RIFs had PCR-SSCP patterns identical to that of H37Rv. The sensitivity of the assay was 31.4%; its specificity was 100%. We observed a strong correlation between the degree of resistance and the type of mutation. *********** In the developed world, tuberculosis (TB), once considered to have been essentially eliminated, has rebounded and is increasingly caused by drug-resistant strains. In developing countries, however, TB has been an unrelenting scourge. Increasing international travel and migration contribute to its widespread dissemination. Consequently, in 1993, the World Health Organization declared TB to be a global emergency (1). Drug-resistant TB is a widespread phenomenon, with primary isoniazid-resistance rates as high as 32% and primary multidrug resistance multidrug resistance, n the adaptation of tumor cells or infectious agents to resist chemotherapeutic agents. close to 15% in the former Soviet Union. In Latin America, primary resistance 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. varies from 1% in Uruguay to 20% in the Dominican Republic, and primary multidrug resistance is as high as 7% in the Dominican Republic and 5% in Argentina (2). In 1995, we reported increasing resistance rates to isoniazid and 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. , four times higher than previously reported rates for Mexico (3). Since then, several studies have addressed this issue in different settings: urban, semi-urban, and rural areas. The common finding has been a high rate of primary resistance to isoniazid and to the combination of isoniazid and rifampin (4,5). In 2000, a collaborative effort between the Centers for Disease Control and Prevention Centers for Disease Control and Prevention (CDC), agency of the U.S. Public Health Service since 1973, with headquarters in Atlanta; it was established in 1946 as the Communicable Disease Center. and the Mexican TB control program reported an 11% rate of primary isoniazid resistance and 2% of primary multidrug resistance (6). From the public health perspective, the impact of resistance on disease and death has recently been emphasized (7) in settings where 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. is highly prevalent. However, its impact is also high in semi-urban settings without the influence of HIV infection (8). Thus, reliable methods are urgently needed to rapidly detect resistance, particularly to rifampin (a marker for multidrug resistance), without cumbersome traditional methods or use of radioactivity (9). Several techniques use 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) )-based strategies to rapidly detect mutations known to confer resistance. One such method is single-stranded conformational polymorphism (SSCP (1) (System Services Control Point) A controlling program in an SNA domain. It resides in the host and is a component within VTAM. See also SCCP. ) analysis, which involves amplification by PCR of a segment of the gene encoding for the specific drug target and comparison of PCR products of drug-sensitive and drug- resistant strains by SSCP, in which mutations usually result in an altered pattern (9,10). This technique is relatively simple and was promising initially, but recent studies have questioned its sensitivity and specificity (10). We investigated the usefulness of PCR-SSCP to detect mutations in the rpoB gene of Mycobacterium tuberculosis strains with a wide range of rifampin resistance and whether specific mutations in this gene are associated with degree of rifampin resistance. Methods Clinical Isolates Forty-six clinical isolates 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. were included in this study; all isolates were recovered from sputum sputum /spu·tum/ (spu´tum) [L.] expectoration; matter ejected from the trachea, bronchi, and lungs through the mouth. sputum cruen´tum bloody sputum. samples of patients from Mexico City and were fully characterized by conventional methods (11). All strains were resistant to at least one primary antituberculosis agent (isoniazid 0.1 [micro]g/mL, rifampin 2 [micro]g/mL, 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 6 [micro]g/mL, or ethambutol ethambutol /etham·bu·tol/ (e-tham´bu-tol) an antibacterial, specifically effective against Mycobacterium; used with one or more other antituberculous drugs in the treatment of pulmonary tuberculosis, administered as the 7.5 [micro]g/mL). Thirty-five strains were rifampin resistant (RIFr), and 11 were rifampin sensitive (RIFs). MICs to the primary antituberculosis drugs Antituberculosis Drugs Definition Antituberculosis drugs are medicines used to treat tuberculosis, an infectious disease that can affect the lungs and other organs. were determined by the radiometric method (Becton Dickinson, Cockeysville, MD) (12). PCR Amplification Chromosomal 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 extracted by conventional methods (13). A 157-bp fragment of the rpoB gene was amplified by PCR with primers Tb8 (5'TGCACGTCGCGG ACCTCCA3') and Tb9 (5'TCGCCGCGATCAAGGAGT3'). PCR was carried out in 50 [micro]L of a reaction mixture containing 50 mM KCl, 10 mM Tris (pH 8.0), 1.5 mM Mg[Cl.sub.2], 100 [micro]m of deoxynucleoside triphosphates (dNTPs), 1U Taq polymerase, 10 pmoles of each set of primers, and 10 ng of chromosomal DNA. Samples were then subjected to one cycle at 94 [degrees] C for 5 min, followed by 40 cycles at 94 [degrees] C for 1 min, 55 [degrees] C for 1 min, 72 [degrees] C for 1 min, and a final cycle at 72 [degrees] C for 8 min to complete the elongation of the PCR intermediate products. PCR products were then run on 2% agarose agarose more highly purified form of agar with similar uses to agar and widely used in the separation of nucleic acid fragments. gels and examined for the presence of the 157-bp band after ethidium bromide staining. Screening of SSCP-PCR Products The SSCP of PCR products was analyzed by electrophoresis with 12% acrylamide acrylamide /acryl·a·mide/ (ah-kril´ah-mid) a vinyl monomer used in the production of polymers with many industrial and research uses; the monomeric form is a neurotoxin. gels. In brief, 25 [micro]L of the amplified product was diluted with 100 [micro]L of buffer (0.1% sodium dodecyl sulfate Sodium dodecyl sulfate (or sulphate) (SDS or NaDS) (C12H25NaO4S),is an anionic surfactant that is used in household products such as toothpastes, shampoos, shaving foams and bubble baths for its thickening effect and its ability to , EDTA EDTA: see chelating agents. 10 mM); 3 [micro]L of this dilution was mixed with 3 [mciro]L of loading buffer (95% formamide, 20 mM EDTA, and 0.05% each of bromophenol blue and xylene cyanol). The mixtures were boiled for 2 min, cooled in ice for 5 min, and then loaded on the gel at 40V for 10 h at room temperature. The gels were silver stained and allowed to dry. The drug-susceptible strain H37Rv was run side by side with the clinical isolates as a control for all experiments. Three different PCR products were analyzed five times each. DNA Sequencing A 411-bp fragment of the rpoB gene, containing the sequence of the 157-bp rpoB fragment, was amplified by PCR using primers TR1 (5' TACGGTCGGCGAGCT GATCC3') and TR2 (5'TACGGCGTTTCGATGAACC3'). PCR was carried out in 25 [micro]L containing 50 mM KCl, 10 mM Tris (pH 8.0), 0.7 mM Mg[Cl.sub.2], 100 [micro]M dNTPs, 1U Taq polymerase, and 10 ng of DNA template. Samples were then subjected to one cycle at 94 [degrees] C for 5 min, followed by 40 cycles at 94 [degrees] C for 1 min, 55 [degrees] C for 1 min, 72 [degrees] C for 1 min, and a final cycle at 72 [degrees] C for 8 min to complete the elongation of the PCR intermediate products. These products were characterized by electrophoresis on 2% agarose gels and stained in 0.5 [micro]g/mL of ethidium bromide. PCR products were sequenced directly on an Applied Biosystems 373A automated DNA sequencer (Perkin Elmer, Foster City, CA). Samples that gave a single band on agarose gels were purified (Wizard PCR Preps, Promega, Madison, WI) to remove excess primers and nucleotides. Sequencing was done with a PRISM dye terminator cycle sequencing kit (Perkin Elmer), following the manufacturer's instructions. Statistical Analysis Sensitivity and specificity of the PCR-SSCP method were determined by using the test for 2X2 contingency tables. Differences in the mean MIC logs among strains with specific mutations were calculated by the two-sample Wilcoxon rank-sum test (Mann-Whitney U test Mann-Whitney U test, n.pr See test, Mann-Whitney U. ). Results Rifr Pattern among M. tuberculosis Isolates The 35 RIFr isolates had MIC values as follows: two isolates had an MIC of 2 [micro]g/mL; six of 8 [micro]g/mL; one of 16 [micro]g/ mL; one 32 [micro]g/mL; two of 64 [micro]g/mL; two of 128 [micro]g/mL; eight of 256 [micro]g/mL; one of 512 [micro]g/mL; two of 1,024 [micro]g/mL, and ten of 2,048 [micro]g/mL. All 11 rifampin-susceptible isolates had MIC values [less than or equal to] 0.5 [micro]g/mL, but all of them were resistant to at least one other primary antituberculosis agent. SSCP Analysis SSCP assays were repeated at least five times with three different amplicons for all isolates with 100% reproducibility. On the basis of the SSCP results, the 35 RIFr isolates were grouped in two main categories: group one, 24 isolates (68.6%) with an SSCP identical to that of the control strain H37Rv, and group two, 11 isolates (31.4%) with an SSCP different from that of H37Rv. The MICs were variable in group one. In group two, four polymorphisms were observed with different MICs (Figure). The 11 RIFs isolates showed an SSCP identical to that of H37Rv. Therefore, the overall sensitivity of the assay was 31.4%, with a specificity of 100%. It was not possible to correlate the MIC values with the polymorphisms because each strain had a different MIC. [FIGURE OMITTED] DNA-Sequencing Analysis No mutations were found in the core region of the rpoB gene in the 11 RIFs isolates. All 35 RIFr isolates showed a mutation by sequence analysis. Seven different missense mutations were observed, with all but one detected within the core region. These mutations produced 13 changes in amino acid amino acid (əmē`nō), any one of a class of simple organic compounds containing carbon, hydrogen, oxygen, nitrogen, and in certain cases sulfur. These compounds are the building blocks of proteins. content (Table). Mutations at specific codons were associated with the level of resistance; significantly higher MICs were observed when point mutations occurred in codon codon: see nucleic acid. 513 (median MIC 2,048 [micro]g/mL; p=0.001), in codon 526 (median MIC 2048 [micro]g/mL, p=0.002), and in codon 531 (median MIC 256 [micro]g/mL, p=0.002), compared with mutations at codon 516 (median MIC 8 [micro]g/mL). Single strains with low-level resistance had mutations at codons 522 (MIC 8 [micro]g/mL), 533 (MIC 2 [micro]g/mL), and 572 (MIC 2 [micro]g/mL) (Table). Three mutations in codon 531 had not been described previously. Neither insertions nor deletions were detected in this group of strains. Discussion PCR-SSCP has been used extensively to search for genetic diseases (14,15) and recently to detect missense mutations associated with antibiotic resistance antibiotic resistance, n the ability of certain strains of microorganisms to develop resistance to antibiotics. antibiotic resistance in M. tuberculosis (9,10,16,17). In spite of extensive and comprehensive standardization of the PCR-SSCP method, our data show that this procedure was highly specific but had poor sensitivity for detecting mutations in the rpoB gene in rifampin-resistant clinical isolates of M. tuberculosis, since two thirds of the resistant isolates had a PCR-SSCP pattern similar to that of the M. tuberculosis susceptible control strain H37Rv. Our results differ from those of the investigators who first tested this technique to detect rifampin resistance in M. tuberculosis and demonstrated a clear association between rpoB mutations and the resistance profile (9). However, in recent studies, this method has detected silent and missense mutations in susceptible strains (18). We did not find these types of mutations, but we did find 24/35 (68.6%) false-negative results. Furthermore, in a recent study by Lee et al. in Korea, false-negative results were obtained in 17 (25.4%) of 67 strains (10). Although suboptimal Suboptimal A solution is called suboptimal if a part of the solution has been optimized without regards to the overall objective. technical conditions may account for the poor PCR-SSCP performance, missense mutations were found after nucleotide sequencing in rifampin-resistant strains. Although the method was fully reproducible, after the data were controlled for all variables, our data also indicate that this method may perform poorly in detecting mutations in this region. To confirm our findings with PCR-SSCP, we determined the nucleotide sequence in 35 rifampin-resistant M. tuberculosis strains and observed missense mutations in all of them (Table). After sequence analysis, all the highly rifampin-resistant ([greater than or equal to] 128 [micro]g/mL) isolates were found to have point mutations in codons 513, 526, and 531, which were the most common in our study population, corroborating that these mutations are the most prevalent worldwide (19). Since our strains showed different types of mutations, we do not endorse the recently suggested idea of a geographic distribution of single mutations (20,21). Additionally, we observed three alleles in codon 531 that had not been described previously: two strains showed an TCG/GCG (Ser/Ala) exchange, one an TCG/CCG (Ser/Pro) exchange, and another an TCG/ TTC TTC Trying To Conceive TTC Toronto Transit Commission TTC Trans Texas Corridor TTC Toutes Taxes Comprises (French) TTC Trident Technical College (North Charleston, SC) TTC Temporary Traffic Control (Ser/Phe) exchange. There was a strong correlation between the degree of resistance and any nucleotide substitution in specific codons. Mutations associated with nucleotide replacements in codons 513, 526, and 531 were associated with high-level rifampin resistance, whereas mutations in codon 516 were observed in low-level rifampin resistance (p<0.005) (Table). Other authors have reported high (22,23) and low (24) levels of resistance associated with specific nucleotide replacements. These differences reflect the complex and crucial interaction between the drug and its target at the molecular level, where the position of the affected 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. seems to be critical. An additional interesting finding was that one strain with an MIC of 2 [micro]g/mL did not show a mutation within the 81-bp core region, although a missense mutation ATC/TTC (Ile/Phe) was seen in codon 572, which may explain the rifampin resistance detected in this strain. This observation confirms a recent report of a rifampin-resistant strain identified in Australia with an identical mutation outside the core region of rpoB (25). Although the SSCP method performed poorly in our setting, other DNA sequence-based approaches to detecting rifampin resistance may still have merit, since the vast majority of mutations occur in precisely defined positions. For example, INNO-LIPA (26) is a promising method based on specific detection of previously identified resistance-conferring mutations. Alternatively, other methods based on cell viability, such as use of mycobacteriophages and reporter genes, have shown promise (27, 28). In conclusion, the practical implications of our study are that the PCR-SSCP method may not be a reliable tool for the detection of resistance to rifampin in M. tuberculosis. However, if our observation of a strong correlation between specific mutations and the level of resistance is confirmed in other settings, the level of rifampin resistance may be predictable by DNA sequence-based resistance detection methods.
Table. Mutations of the rpoB gene found in 35 rifampin-resistant
Mycobacterium tuberculosis isolates
Mutated
rpoB Specific Strain
codon Mutation n
513 CAA/AAA(Gln/Lys) 1
CAA/AAA(Gln/Lys) 1
CAA/CCA(Gln/Pro) 1
516 GAC/GTC(Asp/Val) 5
526 CAC/TAC(His/Tyr) 1
CAC/TAC(His/Tyr) 1
CAC/TAC(His/Tyr) 3
CAC/GAC(His/Asp) 2
CAC/GAC(His/Asp) 1
CAC/GAC(His/Asp) 1
531 TCG/TTG(Ser/Leu) 1
TCG/TTG(Ser/Leu) 1
TCG/TTG(Ser/Leu) 4
TCG/TTG(Ser/Leu) 1
TCG/TTG(Ser/Leu) 3
TCG/CCG(Ser/Pro) (b) 1
TCG/GCG(Ser/Ala) (b) 1
TCG/GCG(Ser/Ala) (b) 1
TCG/TGG(Ser/Trp) 1
TCG/TTC (Ser/Phe) (b) 1
522 TCG/TTG (Ser/Leu) 1
533 CTG/CCG (Leu/Pro) 1
572 ATC/TTC (Ile/Phe) (a) 1
Mutated
rpoB MIC
codon ([micro]g/mL) p (c)
513 2,048 0.01
256 0.01
2,048 0.01
516 37,118 0.01, 0.002
526 256 0.01, 0.002
1,024 0.01, 0.002
2,048 0.01, 0.002
256 0.01, 0.002
128 0.01, 0.002
2,048 0.01, 0.002
531 32 0.002
64 0.002
256 0.002
1,024 0.002
2,048 0.002
8 0.002
64 0.002
128 0.002
512 0.002
2,048 0.002
522 8
533 2
572 2
(a) This mutation is located outside the core region.
(b) Not previously described.
(c) Mann-Whitney test.
Acknowledgments We thank B. Chavez-Mazari and G. Hernandez for technical support. This study was partially supported by grants from CONACyT, G-26264/M, and the Fogarty International Center, FIRCA FIRCA Fogarty International Research Collaboration Award , PA-95-011, NIH "Not invented here." See digispeak. NIH - The United States National Institutes of Health. , ICIDR-5U01AI35969 and ERID-TW-96-001 and UNAM-PADEP (201313). Miriam Bobadilla-del-Valle was a recipient of a CONACyT scholarship (No. 118152). Dr. M. Bobadilla-del-Valle is a molecular microbiologist in the Laboratory of Clinical Microbiology, Instituto Nacional de Ciencias Medicas y Nutricion Salvador Zubiran, Mexico. Her research involves the molecular basis of drug resistance in tuberculosis. References (1.) Pablos-Mendez A, Raviglione MC, Laszlo A, Binkin N, Rieder HL, Bustreo F, et al. Global surveillance for antituberculosis-drug resistance, 1994-1997. N Engl J Med 1998;338:1641-9. (2.) 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Mutation position and type of substitution in the [beta]-subunit of the RNA polymerase influence in-vitro activity of rifamycins in 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. resistant Mycobacterium tuberculosis. J Antimicrob Chemother 1995;35:345-8. (25.) Lilly K, Yuen W, Leslie D, Cole PJ. Bacteriological bac·te·ri·ol·o·gy n. The study of bacteria, especially in relation to medicine and agriculture. bac·te and molecular analysis of rifampin-resistant Mycobacterium tuberculosis strains isolated in Australia. J Clin Microbiol 1999;37:3844-50. (26.) 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. (27.) Jacobs WR Jr, Barletta RG, Udani R. Rapid assessment of drug susceptibilities by means by luciferase luciferase (loosif´  rās´),n an enzyme present in certain luminous organisms that act to bring about the oxidation of luciferins; energy produced in the reporter phages. Science 1993;260:819-22. (28.) Banaiee N, Bobadilla-del-Valle M, Bardarov S, Riska PF, Small PM, Ponce-de-Leon A, et al. Evaluation of luciferase reporter mycobacteriophage technology for detection, identification, and antibiotic susceptibility testing of Mycobacterium tuberculosis complex in Mexico. Abstracts and final program of the 2001 Keystone Symposia on Molecular and Cellular Aspects of Tuberculosis Research in the Post Genome Era (B1). Taos, New Mexico Taos (IPA: [taʊs]) is a town in Taos County in the north-central region of New Mexico. In New Mexico, a municipality may call itself a village, town, or city. . January 25-30, 2001. Abstract 204, p. 69. Miriam Bobadilla-del-Valle, * Alfredo Ponce-de-Leon, * Catalina Arenas-Huertero, * Gilberto Vargas-Alarcon, ([dagger]) Midori Kato-Maeda, * Peter M. Small, ([double dagger]) Patricia Couary, * Guillermo M. Ruiz-Palacios, * and Jose Sifuentes-Osornio * * Instituto Nacional de Ciencias Medicas y Nutricion Salvador Zubiran, Mexico City, Mexico; ([dagger]) Instituto Nacional de Cardiologia Ignacio Chavez and Universidad Panamericana, Mexico City, Mexico; and ([double dagger]) Stanford University Medical Center Stanford University Medical Center (Stanford Hospital & Clinics) is one of four hospitals affiliated with Stanford University and Stanford University School of Medicine, along with the Lucile Packard Children's Hospital, the Veteran's Administration Hospital in Palo Alto, and Santa , Stanford, California, USA Address for correspondence: Jose Sifuentes-Osornio, Departamento de Infectologia, Instituto Nacional de Ciencias Medicas y Nutricion Salvador Zubiran, Vasco de Quiroga Vasco de Quiroga (ca. 1470, Madrigal, Castile—March 14, 1565, Uruapan) was the first bishop of Michoacán, Mexico and one of the judges (oidores) in the second Audiencia that governed New Spain from January 10, 1531 to April 16, 1535. 15, Tlalpan, Mexico 14000 D.F. Mexico; fax: (525) 513-3945; e-mail: jso@quetzal quetzal (kĕtsäl`) or quezal (kāsäl`), common name for a magnificent bird of the family Trogonidae (trogon family), found in the rain forests from S Mexico to Costa Rica at altitudes of up to 9,000 .innsz.mx |
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