当前位置: 首页 > 期刊 > 《抗菌试剂及化学方法》 > 2003年第1期 > 正文
编号:10585871
Molecular Characterization of Quinolone-Resistant Neisseria gonorrhoeae in Hong Kong
http://www.100md.com 《抗菌试剂及化学方法》2003年第1期
     Sexually Transmitted Diseases Laboratory, Public Health Laboratory Centre, Pathology Service, Department of Health, Kowloon, Hong Kong, China|, http://www.100md.com

    Received 12 April 2002/ Returned for modification 20 June 2002/ Accepted 17 September 2002|, http://www.100md.com

    ABSTRACT|, http://www.100md.com

    In Hong Kong, ParC changes among high-level quinolone-resistant Neisseria gonorrhoeae (QRNG) isolates at Ser-87Arg were associated with a higher level of resistance than a Ser-87Ile alteration. Two previously undescribed mutations in clinical isolates occurring in gyrA, conferring Ala-92Pro and Asp-95Tyr changes, were detected. Nine different outer membrane lipoprotein (Lip) repeat classes—11 to 19 repeats—were identified, with repeat lengths of 16 and 17 the most common, indicating considerable strain diversity.|, http://www.100md.com

    TEXT|, http://www.100md.com

    In Hong Kong, a dramatic increase in quinolone-resistant Neisseria gonorrhoeae (QRNG) isolates has been observed (2-4). These made up 24% of our isolates in 1996 and 50% of our isolates in 1998 and then reached a high level of endemicity of 80% in 2000. All N. gonorrhoeae isolates possess an outer membrane lipoprotein, designated Lip, which was first revealed by a monoclonal antibody designated H.8. The protein epitope is immunogenic in humans and conserved among pathogenic Neisseria species, including N. gonorrhoeae and N. meningitidis, but not most nonpathogenic Neisseria species. We report on the current genetic alteration patterns within the quinolone resistance-determining region (QRDR) in GyrA and ParC proteins from organisms with various levels of quinolone resistance in Hong Kong and also examined these strains by Lip subtyping (1) and assessed whether Lip subtyping is useful in a situation in which QRNG isolates are occurring at high levels of endemicity.

    One hundred six clinical strains of N. gonorrhoeae were drawn randomly from isolates obtained consecutively from patients attending government sexually transmitted disease (STD) clinics during the year 2001. These strains were tested by a standard methodology (5) and classified into four categories of ofloxacin susceptibilities: (i) MIC of 8 µg/ml, 27 isolates; (ii) MIC of 2 but 4 µg/ml, 45 isolates; (iii) MIC of 0.125 but <2 µg/ml, 28 isolates; and (iv) MIC of <0.125 µg/ml, 6 isolates. These were grouped according to previously published data, which correlated MIC with treatment outcome (4). Four World Health Organization (WHO) quality assurance strains (GC1, GC4, GC5, and 94G395) and two controls (F28 and F45) from the Centers for Disease Control and Prevention (CDC), Atlanta, Ga., were used because the ofloxacin MICs for these strains are known, although their molecular characters have not been previously described.5i[}*r, 百拇医药

    The amino acid substitutions in GyrA or ParC protein, based on the nucleotide sequences of gyrA and parC gene fragments that include QRDRs of the respective proteins were investigated by methods previously described (8-10). Nucleotide sequencing was performed by a D-rhodamine dideoxynucleotide chain termination method by using the ABI PRISM 310 Genetic Analyzer (Perkin-Elmer, Foster City, Calif.). Sequence compilation and analyses were carried out with DNAstar software programs (DNASTAR, Inc., Madison, Wis.). For alignment, gyrA and parC genes were compared with U08817 and U08907, respectively (T. Deguchi, M. Yasuda, M. Nakano, S. Ozeki, E. Kanematsu, Y. Kawada, T. Ezaki, and I. Saito, Letter, Antimicrob. Agents Chemother. 40:2437-2438, 1996). The lip gene was amplified by PCR after extraction of the chromosomal DNA by DNAzol (Molecular Research Center, Inc., Cincinnati, Ohio). Amplicons were sequenced, and the primers were used as described previously (12). Profiles of known Lip-type patterns, kindly supplied by D. L. Trees (STD Branch, CDC), were used for alignment and analysis.

    Forty-nine percent of patients acquired the strains locally, while the source of contact of the other patients could be traced to other Chinese provinces, including Macau, in 47% of our isolates. A minority of patients originated from the Philippines and Pakistan, which together accounted for 2%, while the source of the remaining 2% was unknown.'y.#&, http://www.100md.com

    Out of 100 isolates, the ofloxacin MIC for 28 isolates was 0.125 µg/ml but 1 µg/ml, while the ofloxacin MICs for 17, 28, 14, and 13 isolates were 2, 4, 8, and 16 µg/ml, respectively. Table 1 shows the frequency distribution of various GyrA/ParC alteration patterns of quinolone-resistant strains against the respective ofloxacin MICs. Isolates for which the ofloxacin MIC was >0.06 but 1 µg/ml had 11 patterns, mainly possessing a single-site alteration in GyrA (64%). Simultaneous mutations at single sites in both gyrA and parC were mainly found in this category. In contrast, isolates for which the ofloxacin MICs ranged from 2 to 16 µg/ml did not possess alterations at a single site in QRDR. They had double and triple mutations in both gyrA and parC. Isolates for which the ofloxacin MIC was >1 µg/ml had 18 patterns, and 2 patterns predominated—GyrA (Ser91Phe, Asp95Gly) with ParC (Ser87Arg) and GyrA (Ser91Phe, Asp95Gly) with ParC() (where represents the QRDR without mutation)—both in ParC, accounting for 24 and 21%, respectively. Isolates with higher-level resistance (MIC of 4 µg/ml) had an increased tendency toward three mutations in gyrA and parC (P < 0.01). The Ser-87Arg alteration in ParC was associated with a higher level of resistance (MIC of 8 µg/ml) (P < 0.001). Two isolates containing the Ser-87Ile substitution displayed the same high level of resistance (MIC of 16 µg/ml). Two new mutations among clinical isolates occurring in gyrA, conferring an Ala-92Pro change (MIC = 2 µg/ml) and Asp-95Tyr (MIC = 4 µg/ml) were detected. Double alterations in both GyrA and ParC were not found, although they have been reported elsewhere (6, 7, 10). Substitutions in parC alone were not found.

    fig.ommitteedo(^7, 百拇医药

    TABLE 1. Distribution of GyrA and ParC alteration patterns against respective ofloxacin MICs for sample isolates from Hong Kong in 2001ao(^7, 百拇医药

    Among the 106 quinolone-susceptible and -resistant isolates, 9 different Lip repeat classes were identified, ranging from 11 to 19 repeats, but repeat length 20 was not found (12). The respective ofloxacin susceptibility categories [i.e., (i) MIC of <0.125 µg/ml, (ii) MIC of 0.125 but <4 µg/ml, and (iii) MIC of 4 µg/ml] belonged to four (13 to 16 repeats), seven (12 to 18 repeats), and nine (11 to 19 repeats) Lip repeat classes, respectively. Repeat lengths of 16 and 17 were the most predominant in the current sample, comprising 23.6 and 25.5%, respectively. Even though they were predominant, they were found distributed in all ofloxacin MIC categories (except for the group for which an ofloxacin MIC was <0.125 µg/ml) as well as with the MICs of the other antibiotics tested, including penicillin, tetracycline, erythromycin, spectinomycin, and ceftriaxone (data not shown). After sequencing, the number of subtypes has been extended to 28 in Hong Kong and up to 48 when the patterns from D. L. Trees (CDC) and the control strain F28 were included. The 14-repeat class was most diversified and consisted of seven subtypes (Tables 2 and 3). The use of Lip protein typing revealed that QRNG isolates are polyclonal in Hong Kong.

    fig.ommitteed3, http://www.100md.com

    TABLE 2. Frequencies of Lip sequence subtypes in Hong Kong isolates in 20013, http://www.100md.com

    fig.ommitteed3, http://www.100md.com

    TABLE 3. Lip subtypes in controls3, http://www.100md.com

    Based on the sequence differences in the repeats that resulted in amino acid alterations, the nine repeat patterns could be further classified into 28 subtypes. There were three subtypes in the proportion of 13:11:1 in the 16-repeat class and three subtypes in the proportion of 25:1:1 in the 17-repeat class as shown in Table 4. Repeat classes 11 and 19 had a low occurrence, and it is probable that these are more conserved during the course of evolution of quinolone resistance, although there is no genetic linkage between lip, gyrA, and parC.3, http://www.100md.com

    fig.ommitteed3, http://www.100md.com

    TABLE 4. Amino acid sequences of subtypes in 16-repeat class and 17-repeat class in Hong Kong isolates3, http://www.100md.com

    A variety of QRDR patterns were present in Hong Kong, and the most prevalent ones were GyrA (Ser91Phe, Asp95Gly) with ParC (Ser87Arg) (25%) and GyrA (Ser91Phe, Asp95Gly) with ParC () (21%) in ParC. In a recent report, the former alteration pattern was also present in a single strain isolated from mainland China (6). Further studies will be needed to compare cross-country differences, as well as longitudinal changes, in QRDR patterns among QRNG strains isolated from different localities in the region.

    Silent mutations in codons 104 (TAT to TAC), 129 (GCG to GCA), and 131 (CTC to CTG) of parC genes were detected. The former two did not occur in the absence of the latter. These silent mutations occurred in 75% of QRNG strains, but there was no association between these mutations and the alterations in QRDR of GyrA and ParC.23fqk, 百拇医药

    The ParC alterations reported to date have occurred in amino acids Gly-85, Asp-86, Ser-87, Ser-88, Glu-91, Ala-92, and Arg-116 (8, 10). The Asp86Asn alteration was the most prominent pattern seen in the Philippines (11). Ser88Pro was more commonly found in Japan (8, 9), while Ser87Ile, which confers high-level resistance (MIC of 16 µg/ml), was reported in Hawaii, the Philippines, and Japan (11, 13; Deguchi et al., Letter). In Hong Kong, since ofloxacin had been used as the first-line drug for a long period of time, and given the large numbers of travelers passing through from other countries, we have now seen the emergence of a wide variety of alterations in N. gonorrhoeae, and types have been identified that are different from those previously described.

    (Part of this work has been presented at the Tenth International Congress on Infectious Diseases, International Society for Infectious Diseases, Singapore, 11 to 14 March 2002.)}kd0, 百拇医药

    ACKNOWLEDGMENTS}kd0, 百拇医药

    We are indebted to the laboratory staff of Sexually Transmitted Diseases Laboratory in the Public Health Laboratory Centre, Department of Health, for their excellent technical support. We also thank the Director of Health, Margaret Chan, for permission to publish this report.}kd0, 百拇医药

    REFERENCES}kd0, 百拇医药

    Cannon, J. G., W. J. Black, I. Nachamkin, and P. W. Stewart. 1984. Monoclonal antibody that recognizes an outer membrane antigen common to the pathogenic Neisseria species but not to most nonpathogenic Neisseria species. Infect. Immun. 43:994-999.}kd0, 百拇医药

    Kam, K. M., K. K. Lo, N. K. Ho, and M. M. Cheung. 1995. Rapid decline in penicillinase-producing Neisseria gonorrhoeae in Hong Kong associated with emerging 4-fluoroquinolone resistance. Genitourin. Med. 71:141-144.

    Kam, K. M., P. W. Wong, M. M. Cheung, N. K. Ho, and K. K. Lo. 1996. Quinolone-resistant Neisseria gonorrhoeae in Hong Kong. Sex. Transm. Dis. 23:103-108.-;zrz9, 百拇医药

    Kam, K. M., K. K. Lo, L. Y. Chong, W. F. Au, P. Y. Wong, and M. M. Cheung. 1999. Correlation between in vitro quinolone susceptibility of Neisseria gonorrhoeae and outcome of treatment of gonococcal urethritis with single-dose ofloxacin. Clin. Infect. Dis. 28:1165-1166.-;zrz9, 百拇医药

    National Committee for Clinical Laboratory Standards. 1998. Performance standards for antimicrobial susceptibility testing: M100-S8. National Committee for Clinical Laboratory Standards, Wayne, Pa.-;zrz9, 百拇医药

    Shultz, T. R., J. W. Tapsall, and P. A. White. 2001. Correlation of in vitro susceptibilities to newer quinolones of naturally occurring quinolone-resistant Neisseria gonorrhoeae strains with changes in GyrA and ParC. Antimicrob. Agents Chemother. 45:734-738.-;zrz9, 百拇医药

    Su, X., and I. Lind. 2001. Molecular basis of high-level ciprofloxacin resistance in Neisseria gonorrhoeae strains isolated in Denmark from 1995 to 1998. Antimicrob. Agents Chemother. 45:117-123.

    Tanaka, M., H. Nakayama, M. Haraoka, T. Saika, I. Kobayashi, and S. Naito. 2000. Susceptibilities of Neisseria gonorrhoeae isolates containing amino acid substitutions in GyrA, with or without substitutions in ParC, to newer fluoroquinolones and other antibiotics. Antimicrob. Agents Chemother. 44:192-195.+\%9r, http://www.100md.com

    Tanaka, M., S. Sakuma, K. Takahashi, T. Nagahuzi, T. Saika, I. Kobay, and J. Kumazawa. 1998. Analysis of quinolone resistance mechanisms in Neisseria gonorrhoeae isolates in vitro. Sex. Transm. Infect. 74:59-62.+\%9r, http://www.100md.com

    Trees, D. L., A. L. Sandul, W. L. Whittington, and J. S. Knapp. 1998. Identification of novel mutation patterns in the parC gene of ciprofloxacin-resistant isolates of Neisseria gonorrhoeae. Antimicrob. Agents Chemother. 42:2103-2105.+\%9r, http://www.100md.com

    Trees, D. L., A. L. Sandul, V. Peto-Mesola, M. R. Aplasca, H. B. Leng, W. L. Whittington, and J. S. Knapp. 1999. Alterations within the quinolone resistance-determining regions of GyrA and ParC of Neisseria gonorrhoeae isolated in the Far East and the United States. Int. J. Antimicrob. Agents 12:325-332.+\%9r, http://www.100md.com

    Trees, D. L., A. J. Schultz, and J. S. Knapp. 2000. Use of neisserial lipoprotein (Lip) for subtyping Neisseria gonorrhoeae. J. Clin. Microbiol. 38:2914-2916.+\%9r, http://www.100md.com

    Trees, D. L., A. L. Sandul, S. W. Neal, H. Higa, and J. S. Knapp. 2001. Molecular epidemiology of Neisseria gonorrhoeae exhibiting decreased susceptibility and resistance to ciprofloxacin in Hawaii, 1991-1999. Sex. Transm. Dis. 28:309-314.(Kai Man Kam Shirley Sin Yee Kam Danny Tze Leung Cheung Viola Wai Na Tung Wai Fun Au and May May Cheu)