Outbreak of Neisseria meningitidis, in Edmonton, Alberta, Canada. (Dispatches).From December 1999 to April 2001, the greater Edmonton region had 61 cases of invasive meningococcal infection, two fatal. The outbreak was due to Neisseria meningitidis Neisseria men·in·git·i·dis n. The bacteria that is the causative agent of cerebrospinal meningitis; meningococcus. Neisseria meningitidis serogroup C, electrophoretic type 15, serotype serotype /se·ro·type/ (ser´o-tip) the type of a microorganism determined by its constituent antigens; a taxonomic subdivision based thereon. se·ro·type n. See serovar. v. 2a. Analysis of the strains showed that 50 of 56 culture-confirmed cases were due to a single clone and close relatives of this clone. This strain had not been previously identified in the province of Alberta dating back to January 1997. ********** Neisseria meningitidis causes outbreaks of disease resulting in severe illness and death. These outbreaks occur in persons in their teens and early twenties; however, in some outbreaks, the very young (<2 years of age) are also severely affected (1). Persons >25 years of age appear to be less affected. North American North American named after North America. North American blastomycosis see North American blastomycosis. North American cattle tick see boophilusannulatus. outbreaks are confined primarily to serogroup C strains and less commonly to Y and W135 (2-5). We report an outbreak of a serogroup C clone of N. meningitidis in the Edmonton region of Alberta, Canada; the serogroup had a unique 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 (RFLP RFLP abbr. restriction fragment length polymorphism RFLP restriction fragment length polymorphism. RFLP ) pattern as determined by pulsed-field gel electrophoresis (PFGE PFGE Pulsed-Field Gel Electrophoresis ). The Outbreak The Edmonton region has a mixed metropolitan and rural population totaling 827,507 (6). From January 1997 to November 1999 (35 months), this region had 13 cases of culture-confirmed invasive N. meningitidis disease (5 from blood, 6 from cerebrospinal fluid [CSF Cerebrospinal Fluid (CSF) Analysis Definition Cerebrospinal fluid (CSF) analysis is a laboratory test to examine a sample of the fluid surrounding the brain and spinal cord. ], and 2 from joints) (Figure 1). Serogroup determination, by the antiserum antiserum /an·ti·se·rum/ (an´ti-se?rum) a serum containing antibody(ies), obtained from an animal immunized either by injection of antigen or by infection with microorganisms containing antigen. agar method previously described, showed that these included two cases of serogroup B, seven of serogroup C, two of serogroup W135, and two of serogroup Y (7,8). During this period, the incidence of culture-confirmed meningococcal disease did not exceed two cases per month (Figure 1). However, from December 1999 to April 2001, 61 cases of invasive N. meningitidis disease occurred; 57 of these were confirmed by culture and 4 on the basis of clinical findings, positive results from an antigen detection assay, or both. The culture-confirmed cases were from blood (51 cases) and CSF (6 cases). Of the 57 culture-confirmed cases, 56 were serogroup C, and 1 was serogroup B (blood isolate). [FIGURE 1 OMITTED] In relation to clinical outcome, 43 (70.5%) of the 61 patients fully recovered; 2 (3.3%) died (a 16-year-old female and a 19-year-old male, both infected with serogroup C) (Figure 1); 4 (6.6%) required amputations; 7 (11.5%) had severe scars; and 9 (14.8%) had other sequelae sequelae Clinical medicine The consequences of a particular condition or therapeutic intervention such as knee pain, neurologic sequelae, decreased hearing, decreased sensation at the extremities, and stiffness in hands. The ages affected during the outbreak period ranged from 5 weeks to 77 years. Outbreak-associated patients were primarily <24 years of age. Age breakdown showed that 10 (17.9%) of 56 confirmed serogroup C strains were in the birth- to 1-year age group (Table). The conjugate vaccine for use in this age group was licensed in Canada in May 2001 and was therefore not available during the outbreak. The high number of cases in this age group translates into an incidence rate of 50 per 100,000 (Table). In comparison, the most recently published national data show the rate for the group <1 year of age to be 12.9/100,000 for 1997 and 6.5/100,000 for 1998 (9). Also, age groups 15-19 and 20-24 showed unusually high incidences of disease in this outbreak (Table). Thirty patients with culture-confirmed disease were female, and 27 were male. Patients were scattered geographically throughout the region, with no more than one case a close contact of another. All contacts of patients were treated with 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. . Except for age group, no particular populations were determined to be at greater risk for infection than other. A vaccination campaign that targeted persons ages 2 to 19 was undertaken in the region from February 14 to 28, 2000, using polysaccharide polysaccharide: see carbohydrate. polysaccharide Any of a large class of long-chain sugars composed of monosaccharides. Because the chains may be unbranched or branched and the monosaccharides may be of one, two, or occasionally more kinds, quadravalent meningococcal vaccine; 168,000 children were immunized. Because of a continuing higher-than-expected number of cases, the vaccine was again offered in October 2000 (Figure 1). This time, the vaccine was offered to all previously unimmunized 2- to 24-year-olds (61,900 doses delivered in 6 days). In April 2001, vaccine was again offered to those 2-year-olds not previously eligible in October 2000. Overall, 87% of people in the targeted age group were vaccinated. After the vaccine campaigns, nine cases of invasive meningococcal disease occurred in those eligible for immunization immunization: see immunity; vaccination. but not immunized (total population of 2- to 24-year-olds 265,300). Nine cases also occurred in the immunized population, for a calculated vaccine effectiveness of 84%. Conclusions Electrophoretic typing, serotyping, and serosubtyping performed by the National Microbiology Laboratory The National Microbiology Laboratory (NML) is located in the Canadian Science Centre for Human and Animal Health in Winnipeg, Manitoba. This modern state-of-the-art facility houses the NML's Biological Safety Level 4 (BSL-4) containment laboratory, currently Canada's only BSL-4 , Population and Public Health Branch of Health Canada, Winnipeg, Canada, showed that all serogroup C strains belonged to electrophoretic type (ET)15, serotype 2a (10). ET15 entered the Canadian population as early as 1986 in Ontario and has since been demonstrated to be responsible for a number of outbreaks in this country (9,11). The most recent data for ETs in Canada date to 1997 and 1998 (9). During 1997, ET15 accounted for 83.1% of strains analyzed. This proportion increased in 1998 to 93.7%, indicating that ET is the predominant type causing invasive disease in Canada. Serosubtyping of serogroup C isolates in this outbreak showed variation in the class 1 outer membrane protein (OMP OMP orotidine 5' monophosphate. OMP decarboxylase enzyme catalyzing the synthesis of uridine monophosphate, the first pyrimidine nucleotide essential for RNA structure. 1). Strains were either P1.2,5 (27 isolates), P1.2 (24 isolates), P1.15 (2 isolates), or P1.-(3 isolates). The two fatal cases were both P1.2,5. Serogrouping, ET, and serosubtyping provided accurate characterization of the circulating strains in the Edmonton region; however, they failed to determine if the outbreak was clonal or if the increased cases were due to unrelated N. meningitidis strains. To determine this, RFLP analysis via PFGE was used with minor modifications (12). Bacterial cells were grown on sheep blood agar. The cells were scraped off and placed in 10% formalin formalin /for·ma·lin/ (for´mah-lin) formaldehyde solution. for·ma·lin n. An aqueous solution of formaldehyde that is 37 percent by weight. for 15 minutes for bacterial inactivation inactivation /in·ac·ti·va·tion/ (in-ak?ti-va´shun) the destruction of biological activity, as of a virus, by the action of heat or other agent. . The cell number was standardized to an optical density of 1.4 at [A.sub.610]. Lysozyme lysozyme: see immunity. Lysozyme An enyme that was first identified and named by Alexander Fleming, who recognized its bacteriolytic properties. was added to 100 [micro]L of cell suspension at a final concentration of 0.2 mg/mL, mixed gently, and added to 1 mL of 1.6% (W/V) low-melting agarose agarose more highly purified form of agar with similar uses to agar and widely used in the separation of nucleic acid fragments. . The mixture was then transferred to the gel plug mold. The gel plug was suspended in Lysis lysis /ly·sis/ (li´sis) 1. destruction or decomposition, as of a cell or other substance, under influence of a specific agent. 2. mobilization of an organ by division of restraining adhesions. 3. II solution (1 mg/mL lysozyme, 0.5% Brij 35, 0.2% sodium deoxycholate, and 0.5% sodium lauryl sarcosine sar·co·sine n. An amino acid made synthetically or formed naturally during the decomposition of creatine. in Tris-EDTA buffer) for 1 hour at 37 [degrees] C, replaced with ESP (1) (Enhanced Service Provider) An organization that adds value to basic telephone service by offering such features as call-forwarding, call-detailing and protocol conversion. buffer (0.25 M EDTA EDTA: see chelating agents. , pH 8.0, 1% sodium lauryl sarcosine, 0.5 mg/mL Proteinase proteinase /pro·tein·ase/ (pro´ten-as?) endopeptidase. pro·tein·ase n. A protease that begins the hydrolytic breakdown of proteins usually by splitting them into polypeptide chains. K), and incubated at 50 [degrees] C for 2 hours. Slices of plug (1X5 mm) were digested by using 30 U of the restriction endonuclease enzyme SpeI (GIBCO GIBCO Grand Island Biological Company (tissue culture media enterprise) BRL BRL In currencies, this is the abbreviation for the Brazilian Real. Notes: The currency market, also known as the Foreign Exchange market, is the largest financial market in the world, with a daily average volume of over US $1 trillion. , Burlington, Ontario, Canada) for 2.0 hours. The restricted 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 resolved by PFGE with the following running conditions: initial switch time: 5.0 seconds, final switch time: 25 seconds at 6 V/cm with included angle at 120 [degrees] C for 19 hours. The gel was stained with ethidium bromide. Analysis was performed by using the BioRad Gel Doc System (Bio-Rad Laboratories, Mississauga, Ontario) and Molecular Analyst Software (Bio-Rad). RFLP pattern numbers were assigned to each isolate with one band difference in the RFLP profile. RFLP analysis showed 15 distinguishable patterns (Figure 2A). Five of these RFLP patterns were seen only from January 1997 to November 1999 (patterns 6, 17, 20, 21, and 22). These patterns were identified by retrospectively determining their RFLP profile from archived strains. The remaining 10 were present only from December 1999 to April 2001 (patterns 3, 7, 8, 11, 12, 16, 25, 32, 34, and 44). Figure 2B shows a dendro-gram analysis of the 15 Spe I-generated RFLP profiles generated by using a 1% tolerance. We used an 85% breakpoint The location in a program used to temporarily halt the program for testing and debugging. Lines of code in a source program are marked for breakpoints. When those instructions are about to be executed, the program stops, allowing the programmer to examine the status of the program to determine relatedness, as reported by Popovic et al. (13). At the 85% relatedness breakpoint, the RFLP profiles formed seven clusters. RFLP patterns for the largest cluster (49 isolates-cluster 4) were only seen during the outbreak period (December 1999 to April 2001). Both deaths were associated with RFLP pattern 3 strains. Interestingly, pattern 7 in cluster 3 was similar on visual examination to pattern 3 (Figure 2A). The first RFLP pattern (first case) detected was pattern 3 (December 24, 1999) followed by pattern 7 (second case, December 29, 1999). Pattern 7 was not detected before December 1999. These data suggest that patterns 3 and 7 arose concomitantly. Even though these patterns appear close in time, pattern 3 and its relatives resulted in 51 cases, whereas pattern 7 was isolated from only 3 cases. Whether pattern 3 strains are more virulent than pattern 7 strains remains to be determined. We have also received reports that this clone has caused disease in other regions of the province of Alberta and in one other Western Canadian province in the same period reported for our outbreak. [FIGURE 2 OMITTED] In conclusion, the Edmonton region in the province of Alberta, Canada, had an outbreak of N. meningitidis caused by a clone unique to this region. This clone was associated with increased deaths and can readily spread beyond defined geographic boundaries. Other provincial and state laboratories need to be able to recognize this clone should it appear in their area.
Table. Rates of Neisseria meningitidis disease in the Edmonton, Alberta
Canada, region (per 100,000) (a)
Age (cases)
Rate [less than or 2-4 5-9 10-14
equal to] 1
17-month period (b) 50.0 (9) 9.7 (3) 5.3 (3) 6.8 (4)
Annualized 37.5 7.3 4.0 5.1
Age (cases)
Rate 15-19 20-24 25-34 35-59
17-month period (b) 35.7 (20) 10.6 (6) 4.0 (5) 2.3 (7)
Annualized 26.8 8.0 3.0 1.8
Age (cases)
Rate [greater than or
equal to] 60
17-month period (b) 1.7 (3)
Annualized 1.3
(a) Population=827,507 (6).
(b) December 1999 through April 2001.
Acknowledgments We thank Jan Stoltz and Raymond Tsang for providing the electrophoretic typing, subtyping, and serosubtyping analysis, and Susanna Schmink for providing Neisseria meningitidis strain CDC See Control Data, century date change and Back Orifice. CDC - Control Data Corporation 413. Dr. Tyrrell is a clinical microbiologist in the Provincial Laboratory for Public Health-Alberta. He holds academic appointments in the Departments of Laboratory Medicine and Pathology and Medical Microbiology and Immunology, University of Alberta. He is also the Director of the National Centre for Streptococcus-Canada. His research interests are streptococci Streptococcus (plural, streptococci) A genus of spherical-shaped anaerobic bacteria occurring in pairs or chains. Sydenham's chorea is considered a complication of a streptococcal throat infection. and meningococci. References (1.) Jackson LA, Schuchat A, Reeves MW, Wenger JD. Serogroup C meningococcal outbreaks in the United States, an emerging threat. JAMA JAMA abbr. Journal of the American Medical Association 1995;273:383-9. (2.) Schwartz B, Moore PS, Broome CV. The global epidemiology of meningococcal disease. Clin Microbiol Rev 1989;2:S118-S124. (3.) Tikhomirov E. Meningococcal meningitidis: global situation and control measures. World Health Stat Q 40:98-108. (4.) Achtman M. Molecular epidemiology of epidemic meningtidis. Rev Med Microbiol 1990;1:29-38. (5.) Apicella MA. Neisseria meningitidis, In: Mandel GL, Bennet JE, Dolin R, editors. Principles and practice of infectious diseases. 5th ed. Philadelphia: Churchill Livingstone; 2000. p. 2228-41. (6.) Predy GN, Lightfoot P, Edwards J, Fraser-Lee N. How healthy are we? Health status in the Capital Health Region-A technical report 2000. Edmonton, Alberta: Capital Health Authority; 2001. (7.) Ashton FE, Ryan A, Diena BB. Improved antiserum agar for the serogroup differentiation of Neisseria meningtiditis Y and w135. Can J Microbiol 1980;26:630-2. (8.) Craven DE, Frasch EE. Serogroup identification of meningococci by a modified antiserum agar method. J Clin Microbiol 1979;9:547-8. (9.) Squires SG, Pelletier L, Mungai M, Tsang R, Collins F, Stoltz J. Invasive meningococcal disease in Canada, 1 January 1997 to 31 December 1998. Can Commun Dis Rep 2000;26-21:177-82. (10.) Abdillahi H, Poolman JT. Whole-cell ELISA ELISA (e-li´sah) Enzyme-Linked Immuno-Sorbent Assay; any enzyme immunoassay using an enzyme-labeled immunoreactant and an immunosorbent. ELISA n. for typing Neisseria meningitidis with monoclonal antibodies. FEMS Microbiol Lett 1987;48:36771. (11.) Ashton FE, Ryan JA, Borczyk A, Caugant DA, Mancino L, Huang D. Emergence of a new virulent clone of Neisseria meningitidis serotype 2a that is associated with meningococcal group C disease in Canada. J Clin Microbiol 1991;29:2489-93. (12.) Chang N, Chui L. A standardized protocol for the rapid preparation of bacterial DNA for pulsed-field electrophoresis. Diagn Microbiol Infect Dis 1998;31:275-9. (13.) Popovic T, Schmink S, Rosenstein NA, Ajello GW, Reeves MW, Plikaytis B, et al. Evaluation of pulsed-field gel electrophoresis in epidemiological investigations of meningococcal disease outbreaks caused by Neisseria meningitidis serogroup C. J Clin Microbiol 2001;39:75-85. Address for correspondence: Gregory J. Tyrrell, Room 2B3.13 Walter Mackenzie Centre, The Provincial Laboratory for Public Health for Alberta, 8440-112 Street, Edmonton, Alberta T6G 2J2; fax: 780-407-3864; e-mail: g.tyrrell@provlab.ab.ca Gregory J. Tyrrell, * ([dagger]) Linda Chui, * Marcia Johnson, ([double dagger]) Nicholas Chang, * Robert P. Rennie, * ([dagger]) James A. Talbot, * ([dagger]) and The Edmonton Meningococcal Sturdy Group (1) * The Provincial Laboratory of Public Health for Alberta, Alberta, Canada; ([dagger]) The University of Alberta, Edmonton, Alberta, Canada; ([double dagger]) The Capital Health Authority, Edmonton, Alberta, Canada (1) The Provincial Laboratory of Public Health for Alberta; Dora Lee, The Capital Health Authority; Kari Bergstrom, Gerald Predy, Alberta Health and Wellness; Karen Grimsrud, Agnes Honish, and John Waters. |
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