Serologic response to culture filtrate antigens of Mycobacterium ulcerans during Buruli ulcer disease.Buruli ulcer (BU) is an emerging necrotic skin disease caused by Mycobacterium ulcerans. To assess the potential for a serodiagnostic test, we measured the humoral immune response humoral immune response The immune response involving the transformation of B cells into plasma cells that produce and secrete antibodies to a specific antigen. See Note at antibody. Noun 1. of BU patients to M. ulcerans antigens and compared this response with delayed-type hypersensitivity hypersensitivity, heightened response in a body tissue to an antigen or foreign substance. The body normally responds to an antigen by producing specific antibodies against it. The antibodies impart immunity for any later exposure to that antigen. responses to both Burulin and PPD (1) (Parallel Presence Detect) The method used by earlier SIMM memory modules to communicate their capacity to the computer. A binary number coming from a parallel set of pins was read by the system, with each pin representing one bit. Contrast with SPD. . The delayed-type hypersensitivity response generally supported the diagnosis of BU, with overall reactivity to Burulin in 28 (71.8%) of 39 patients tested, compared with 3 (14%) of 21 healthy controls. However, this positive skin test response was observed primarily in patients with healed or active disease, and rarely in patients with early disease (p=0.009). When tested for a serologic se·rol·o·gy n. pl. se·rol·o·gies 1. The science that deals with the properties and reactions of serums, especially blood serum. 2. response to M. ulcerans culture filtrate filtrate /fil·trate/ (fil´trat) a liquid or gas that has passed through a filter. fil·trate v. To put or go through a filter. n. , 43 (70.5%) of 61 BU patients had antibodies to these antigens, compared with 10 (37.0%) of 27 controls and 4 (30.8%) of 13 tuberculosis patients. There was no correlation between disease stage and the onset of this serum antibody response. Our findings suggest that serologic testing may be useful in the diagnosis and surveillance of BU. Buruli ulcer (BU) disease,, caused by Mycobacterium ulcerans, is characterized by severe necrotizing necrotizing /nec·ro·tiz·ing/ (nek´ro-tiz?ing) causing necrosis. Necrotizing Causing the death of a specific area of tissue. Human bites frequently cause necrotizing infections. ulcers. The disease, which is found worldwide but primarily in tropical climates (1,2), occurs predominantly in children ages 5 to 14 (3) and is associated with severe illness and permanent disabilities in [is greater than] 26% of patients (1,3). Over the past decade, the incidence of BU disease has dramatically increased in several West African countries, notably Ghana, Cote d'Ivoire, Benin, and Togo (1,2). In some West African communities, BU has replaced tuberculosis (TB) and leprosy leprosy or Hansen's disease (hăn`sənz), chronic, mildly infectious malady capable of producing, when untreated, various deformities and disfigurements. as the most prevalent mycobacterial mycobacterial emanating from or pertaining to mycobacterium. mycobacterial granuloma may be caused by Mycobacterium tuberculosis (see cutaneous tuberculosis), M. disease, affecting up to 22% of the population (4). However, the true global impact of the disease is unknown because reliable tools for its rapid diagnosis and surveillance are lacking. In addition, neither the mode of transmission nor the environmental reservoir for M. ulcerans is known, although observational studies suggest that M. ulcerans infection is transmitted through the skin after contact with contaminated water, vegetation (5), or insects (6). Current treatment for cutaneous cutaneous /cu·ta·ne·ous/ (ku-ta´ne-us) pertaining to the skin. cu·ta·ne·ous adj. Of, relating to, or affecting the skin. Cutaneous Pertaining to the skin. disease is primarily surgical. Ulcerative ulcerative /ul·cer·a·tive/ (ul´se-ra?tiv) (ul´ser-ah-tiv) pertaining to or characterized by ulceration. ulcerative pertaining to or characterized by ulceration. lesions require wide debridement Debridement Definition Debridement is the process of removing nonliving tissue from pressure ulcers, burns, and other wounds. Purpose Debridement speeds the healing of pressure ulcers, burns, and other wounds. and skin grafting in specialized health-care facilities, long hospital stays (7), and increased cost to the health-care system and the community (7). Antibiotics are ineffective once ulcers are present, possibly because M. ulcerans is absent from lesions or subcutaneous tissues have already been destroyed, preventing penetration of antimycobacterial drugs (3). Antimicrobial therapy has not been studied in preulcerative lesions because apparently patients rarely visit primary health-care providers with painless nodular nodular marked with, or resembling, nodules. nodular dermatofibrosis see dermatofibrosis. nodular episcleritis see nodular fasciitis (below). nodular fasciitis a firm painless nodular swelling, 0. lesions and diagnostic tests are not available to clearly identify M. ulcerans infection before it progresses to clinical disease. Early identification and surgical excision of these preulcerative nodular lesions can be curative and does not require inpatient care (8). We investigated the serologic response to the M. ulcerans culture filtrate (MUCF) of BU patients at different stages of disease to determine whether serodiagnosis serodiagnosis /se·ro·di·ag·no·sis/ (-di?ag-no´sis) diagnosis of disease based on serologic tests.serodiagnos´tic se·ro·di·ag·no·sis n. pl. is feasible as a tool for early diagnosis and intervention of BU disease. The Study BU patients were identified through a case-control study conducted in 1991 in the Daloa region of Cote d'Ivoire (3). Patients with early ulcerative BU were identified by small, painless, or minimally painful nodules Nodules A small mass of tissue in the form of a protuberance or a knot that is solid and can be detected by touch. Mentioned in: Leprosy or edema edema (ĭdē`mə), abnormal accumulation of fluid in the body tissues or in the body cavities causing swelling or distention of the affected parts. , or ulcerative lesions for [is less than] 2 weeks. Patients with ulcerative BU were identified by lesions that were chronic ([is greater than] 2 weeks duration), were painless or minimally painful, or had undermined edges. Patients with healed BU were identified by stellate stellate /stel·late/ (stel´at) star-shaped; arranged in rosettes. stel·late or stel·lat·ed adj. Arranged or shaped like a star; radiating from a center. scars with retraction in areas of prior ulceration. Descriptive and clinical data were obtained from all BU patients and controls (3). Blood specimens were collected from 82 BU patients and 164 healthy controls in the Daloa region. Because TB is endemic in many of the areas where BU occurs, 13 TB patients from the United States were used as controls for cross-reactivity to MUCF. Use of sera from these patients ensured the lowest probability for exposure to M. ulcerans, so that only cross-reactivity to antigens common to both M. tuberculosis and M. ulcerans would be measured. TB patients were identified through an ongoing study in Atlanta by clinical presentation, a positive PPD response, and isolation of M. tuberculosis from sputum. All specimens tested negative for 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. and were strongly reactive to many of the culture filtrate antigens from M. tuberculosis (data not shown). Informed consent was obtained for all participants, and protocols were approved by the Institutional Review Boards of 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 Ministry of Health of Cote d'Ivoire for the BU study and the Institutional Review Board at Emory University for the TB study. Skin Testing During sera collection, Burulin (9) and PPD (purified protein derivative purified protein derivative see purified protein derivative of tuberculin. of M. tuberculosis, Connaught Laboratories, U.K.) were administered intradermally in·tra·der·mal adj. Within or between the layers of the skin: an intradermal injection. in into the flexor flexor /flex·or/ (flek´ser) 1. causing flexion. 2. a muscle that flexes a joint. flexor retina´culum see entries under retinaculum. surface of the forearms of 39 BU patients and 21 controls, and the diameter of induration induration /in·du·ra·tion/ (in?du-ra´shun) 1. sclerosis or hardening. 2. hardness. 3. an abnormally hard spot or place. was recorded at 48 and 72 hours. The criterion for using Burulin and PPD dual testing to confirm clinical cases of BU has been reported (3,9), and the cumulative delayed-type hypersensitivity (DTH (Direct-To-Home) Typically refers to satellite TV broadcasting directly to a dish antenna on the roof of a house. See DBS. ) findings for this study have been described (Table 1) (3). Sera were also tested for reactivity to MUCF antigen by Western blot (Table 2). [TABULAR DATA 1 NOT REPRODUCIBLE IN ASCII ASCII or American Standard Code for Information Interchange, a set of codes used to represent letters, numbers, a few symbols, and control characters. Originally designed for teletype operations, it has found wide application in computers. ] Table 2. Serologic and skin test responses of Buruli ulcer patients and healthy controls from the villages Clinical presentation Total Burulin (+)(a) AB to MUCF(b) Total BU patients (n = 39) 28 (71.8) 26 (66.7) (%) Healed (n = 16) 15 (93.8) 11 (68.8) (%) Ulcerative (n = 17) 11 (64.7) 11 (64.7) (%) Early ulcerative (n = 6) 2 (33.4) 4 (66.7) (%) No scar or ulcer (n = 21) 3 (14.3) 7 (33.3) (%) (a) Total Burulin (+) numbers and (%) are derived from columns one and two of Table 1 added tog without regard to PPD status, and thus represent the highest possible number (percentage) of [ILLEGIBLE TEXT] BU patients. (b) MUCF = Mycobacterium ulcerans culture filtrate. (c) Denotes all BU patients and controls with any antibodies detected by Western blot analysis West·ern blot analysis n. An electrophoretic procedure for separating proteins. against MUCF. Preparation of MUCF Antigen for Serologic Analysis M. ulcerans strain S-WT (from the Centers for Disease Control and Prevention culture collection; Atlanta) was recovered from a 1-ml lyophilisate in 10% glycerol glycerol, glycerin, glycerine, or 1,2,3-propanetriol (prō`pāntrī'ŏl), CH2OHCHOHCH2OH, colorless, odorless, sweet-tasting, syrupy liquid. by incubation in 5 ml Middlebrook 7H9 with OADC OADC Oregon Association of Defense Counsel OADC Oklahoma Association of Defense Counsel OAdC Originating Address Code (SMS messaging) OADC Ohio Administrative District Council supplement (Remel, Lenexa, KS) at 32.5 [degrees] C for 7 days. This 5-ml inoculum inoculum /in·oc·u·lum/ (-ok´u-lum) pl. inoc´ula material used in inoculation. in·oc·u·lum n. pl. was passaged into 25 ml Middlebrook 7H9 broth supplemented with tryptose and glucose (7H9TG; 0.1% wt:vol and 2% wt:vol, respectively) and incubated at 32.5 [degrees] C for 10 days, followed by passage into 100 ml of 7H9TG and growth at 32.5 [degrees] C for 10 days. Cultivation in this protein- and serum-free media allowed isolation and analysis of specific secreted mycobacterial proteins. The 100-ml culture was passaged into 1L of 7H9TG, incubated at 32.5 [degrees] C in 850-[cm.sup.2] roller bottles, and rotated at 90 rotations per hour. Bacilli were harvested during mid-log phase growth by centrifugation. The 1L of MUCF, containing mycobacterial proteins of interest, was concentrated at 4 [degrees] C under [N.sub.2] by using a stirred-cell apparatus (Amicon Inc., Beverly, MA) with a 10-kDa molecular weight membrane. MUCF was exchanged into 0.1 M [NH.sub.4][HCO HCO Harvard College Observatory HCO Hubbard Communications Office (Scientology) HCO Hearing Carry-Over HCO Health Care Organization HCO Helicopter Control Officer HCO Human Capital Office .sub.3] by dialysis, lyophilized ly·oph·i·lize tr.v. ly·oph·i·lized, ly·oph·i·liz·ing, ly·oph·i·liz·es To freeze-dry (blood plasma or other biological substances). [lyophil(ic) + -ize. , and purified by separation of residual small molecular weight contaminants from antigens of interest by size exclusion chromatography Size exclusion chromatography (SEC) is a chromatographic method in which particles are separated based on their size, or in more technical terms, their hydrodynamic volume. It is usually applied to large molecules or macromolecular complexes such as proteins and industrial polymers. . MUCF was loaded onto a fast-performance liquid chromatography system (FPLC FPLC Franklin Pierce Law Center FPLC Fast Protein Liquid Chromatography (a pharmacia product line) FPLC Fire Place FPLC Fixed-Path Least Congestion (path assignment algorithm) ) (Pharmacia, Piscataway, NJ) equipped with a G-25 superfine superfine a class of merino sheep with wool finer than that of fine-wool. Usual limit is wool of 18.5 microns or less fiber diameter. Sephadex desalting column (Pharmacia, Piscataway, NJ), UV monitor, and conductivity monitor for separation and detection of proteins and salts, respectively. MUCF was eluted with an isocratic gradient of 0.1 M [NH.sub.4][HCO.sub.3]. MUCF protein was quantitated by bicinchoninic acid assay The bicinchoninic acid assay (also known as the BCA assay or Smith assay) is a biochemical assay for determining the total level of protein in a solution, similar to Lowry protein assay, Bradford protein assay or biuret reagent. (Pierce Chemical Co., Rockford, IL) and lyophilized until needed. Approximately 5 mg of MUCF protein was obtained per liter of culture. Aliquots of 8 g of MUCF protein were resolved by discontinuous sodium dodecylsulfate polyacrylamide gel electrophoresis polyacrylamide gel electrophoresis n. A technique for determining the molecular weight of proteins, in which proteins that have been coated in an anionic detergent undergo electrophoresis in a polyacrylamide gel. (SDS-PAGE SDS-PAGE sodium dodecyl sulfate-polyacrylamide gel electrophoresis. ) (10) by using 10% to 20% gradient 10-well gels (Novex, San Diego, CA). MUCF proteins were visualized by staining with silver (11), and this profile was reexamined throughout these experiments to ensure that the MUCF proteins did not degrade upon storage; no antigen variability was seen during our studies. 7H9TG media alone processed in the same way contained no proteins by silver stain analysis after SDS-PAGE and bicinchoninic acid assay. Amino Acid Sequence Analyses The N-terminal amino acid sequences of MUCF proteins were determined and compared with known mycobacterial sequences. One hundred micrograms of MUCF protein was resolved by two-dimensional gel electrophoresis Two-dimensional gel electrophoresis, abbreviated as 2-DE or 2-D electrophoresis, is a form of gel electrophoresis commonly used to analyze proteins. Mixtures of proteins are separated by two properties in two dimensions on 2D gels. (2D-GE) by the method of O'Farrell (12) with the modifications of Sonnenberg and Belisle for resolution of mycobacterial proteins (13). 2D-GE resolved proteins were transferred to 0.1 mm polyvinyl polyvinyl /poly·vi·nyl/ (-vi´nil) a polymerization product of a monomeric vinyl compound. polyvinyl alcohol see under alcohol. difluoride (PVDF PVDF polyvinylidene difluoride ) membrane (14) and visualized by staining with 0.5% Coomassie blue R250 in 40% methanol/10% acetic acid for 2 minutes. The N-terminal amino acid sequence was obtained by loading membranes containing the excised spot of interest onto a Procise-cLC automated Edman 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. (Applied Biosystems, Foster City, CA) and reading the generated chromatographs against amino acid standards. Statistical Analyses Statistical analyses were done by the Mantel-Haenszel chi-square method. Statistical significance for the chi-square p values and Fisher's exact p values was evaluated at [Alpha] = 0.05 Fisher's exact p value was used when the expected cell count was [is less than] 5. Odds ratios (OR) were determined by calculating the ratio of the odds of exposure among cases to that among controls. The test for specificity was determined by dividing the true negatives (n = 24; disease-negative and 70 kDa-negative) by the total number of controls (n = 27). All analyses were done on BU patients and healthy controls from the Daloa region of Cote d'Ivoire, Where the disease is endemic, unless otherwise specified. All data were analyzed by using Exact 2.0b software (D. Martin and H. Austin, Atlanta, GA). Results Seventeen (43.6%) of the 39 skin-tested BU patients had induration of [is greater than or equal to] 10 mm within 72 hours of Burulin administration, with PPD induration at least 3 mm smaller than that with Burulin (Table 1). Only 3 (14.3%) of the 21 skin-tested healthy controls from the area had a similar DTH pattern (Table 1). In addition, 11 (28.2%) of the 39 BU patients had an equally strong response to Burulin and PPD, which suggests that Burulin skin testing may not be reliable in regions where BU and TB are endemic and BCG BCG bacille Calmette-Guérin. BCG abbr. 1. bacillus Calmette-Guérin 2. ballistocardiogram BCG, n.pr See bacille Calmette-Guórin. vaccination is widely used (Table 1). Dual-positive responses included, 28 (71.8%) of the 39 BU patients were Burulin positive. However, when this total Burulin-positive population was delineated by disease stage, positive responses were observed in most of the patients with healed (93.8%) and ulcerative disease (64.7%), but in few (33.4%) patients with early ulcerative disease (Table 2). When healed and active Burulin responses were compared with the DTH response seen in early ulcerative BU patients, a significant difference between the disease stages was found (Fisher's exact p = 0.009). These skin-tested BU patient and control populations from the Daloa region were then tested for reactivity of their sera to MUCF by Western blot, and Burulin induration was compared with serum antibody response (Table 2). Twenty-six (66.7%) of the 39 skin-tested BU patients had an antibody response to the MUCF, versus 7 (33.3%) of the 21 skin-tested controls (chis-quare p = 0.014). BU patient populations had approximately the same positive antibody responses to the MUCF, regardless of disease stage. Specifically, 68.8% of the healed patients were antibody positive, with active ulcerative disease at 64.7% and early disease at 66.7% (Table 2). When the antibody responses of healed and active patients were compared with those seen in early BU patients,, the serologic response did not differ significantly by disease stage (Fisher's exact p = 0.999). Therefore, serologic testing may be useful in the early diagnosis and surveillance of BU. The antibody response to the MUCF was then determined for all 61 clinically diagnosed BU patients and 27 healthy controls, and antibody reactivity to individual antigens was recorded. Three M. ulcerans antigens of 70, 38/36, and 5 kDa were commonly recognized by BU patient sera antibodies (Figure). The 36-kDa antigen was found to be a degradation product of the 38-kDa antigen (unpub. results). Forty-three (70.5%) of 61 BU patient sera had antibodies to at least 1 of 3 antigens, compared with 10 (37.0%) of 27 sera from healthy controls from the area and 4 (30.8%) of 13 sera from TB patients (Table 3). The antibody response to the 70-kDa M. ulcerans antigen was associated with BU disease (OR = 12.33; chi-square p = 0.00002), and the response to this protein was consistent throughout early to late disease stage (OR = 12.4; chi-square p = 0.0000001; Table 3). Results were similar for the 38/36-kDa antigen (OR = 5.94; chi-square p = 0.0016), regardless of disease stage (OR = 3.00; chi-square p = 0.0026). The N-terminal amino acid sequence of the 38 kDa protein was DPAPAPAPRD, and had mycobacterial sequences that precede glycosylation sites (15). The serologic response to the 5-kDa antigen, although common in the seroreactive specimens tested, did not differ significantly between BU patients and healthy controls from disease-endemic areas or TB patients (chisquare p = 0.764 and Fisher's exact p = 0.999, respectively); nor were antibodies to this antigen observed in BU patients at the early ulcerative stage (Table 3). A cross-reactive serologic response to MUCF was observed in some TB patients who had not been exposed to M. ulcerans and in some healthy controls from disease-endemic areas (Figure; representative sample and Table 3). These positive responses may be due to exposure to other mycobacterial pathogens with similar antigens as M. ulcerans or BU disease undetectable by clinical diagnosis, respectively. [TABULAR DATA 3 NOT REPRODUCIBLE IN ASCII] Conclusions Diagnosis of BU currently relies on the clinical presentation of the ulcerative disease stage, by which time the infection has already caused damage, therapeutic options are limited, and outcome is associated with severe disease (3,7,8). Preulcerative nodules and edemous lesions, when identified, frequently contain numerous extracellular mycobacteria mycobacteria members of the genus Mycobacterium. anonymous mycobacteria see opportunist (atypical) mycobacteria (below). nontubercular mycobacteria see opportunist (atypical) mycobacteria (below). (1,2). Thus, diagnosis of BU disease at this early stage may lead to more effective treatment. Indeed, diagnosis of preulcerative BU disease is associated with a better therapeutic outcome and reduced illness (8), and accurate surveillance at the preulcerative stage would enable assessment of the prevalence and global impact of BU disease. Surveillance may also identify risk factors as well as prevention strategies for BU. Consistent with previous reports (3,9), DTH to Burulin, a crude preparation of M. ulcerans lysate ly·sate n. The cellular debris and fluid produced by lysis. (9), was observed in many (71.8%) of the clinically diagnosed BU patients. This overall response was similar to the well-defined cell-mediated DTH responses reported for other mycobacterial infections (16-18), including M. tuberculosis (19,20). In contrast, in BU patients, the Burulin response was associated with ulcerative and healed disease, but not with early ulcerative disease. Thus, unlike other DTH-based monitoring programs that indicate mycobacterial infection before and during disease in immunocompetent im·mu·no·com·pe·tent adj. Having the normal bodily capacity to develop an immune response following exposure to an antigen. im persons, Burulin testing may be more useful for confirming ulcerative disease or monitoring past disease with M. ulcerans in conjunction with PPD results. The marked shared reactivity to PPD and Burulin antigens by BU patients, as measured by similar induration upon intradermal injection, was expected to some degree, considering the commonality of antigenic lipids on the mycobacterial surface, genetic relatedness of mycobacterial pathogens, opportunity of exposure to both mycobacterial pathogens and environmental mycobacteria, and rate of BCG vaccination in the region. When Burulin-positive results were analyzed in conjunction with either the presence of a BCG vaccination scar or recollection of BCG vaccination, 12 of 14 BCG vaccinated BU patients were Burulin positive, and 6 of these 12 patients were also PPD positive. Additionally, all the Burulin- and PPD-positive controls either recalled BCG vaccination or had a BCG scar (data not shown). We found that a specific response to the MUCF was observed in BU patient sera, but unlike the Burulin DTH response, the antibody response did not correlate with disease stage (Table 2). The antibody reactivity in the sera from some of the controls from disease-endemic areas may reflect preclinical infection with M. ulcerans or exposure to other mycobacteria and cross-reactivity to antigens common to mycobacterial species. Interestingly, 10 (55.6%) of the 18 antibody-negative BU patients, versus 15 (33%) of the 43 antibody-positive BU patients, recalled or had a BCG vaccination scar, which suggests that BCG vaccination did not contribute to the antibody response of BU patients to MUCF (data not shown). Thirty percent of the TB patient sera were reactive to MUCF, with reactivity principally towards lower molecular weight proteins and not the 70- or 38/36-kDa proteins (Figure; Table 3). N-terminal amino acid sequence of one of these lower molecular weight proteins, a 31-kDa protein, was found to be FSRPGLPVEY and demonstrated homology with the mycolyl transferases found in M. tuberculosis and other mycobacteria (21). Thus, reactivity of the TB patient sera based on antibodies generated against common mycobacterial antigens is, the likely explanation for the few TB patient sera reactive to MUCF. Our preliminary results indicate the usefulness of the MUCF in detecting BU; specifically, individual antigens in the MUCF may be used for the development of a sensitive and specific test for BU (Table 3). Both the 70- and 38/36-kDa proteins were indicators of BU disease, and antibody responses to both of these proteins were similarly present in BU-reactive patient serum samples, regardless of disease stage. In addition, reactivity to the 70-kDa protein was specific for M. ulcerans infection (88.8%). The 70- and 38/36-kDa proteins may be useful for the development of a serologic test for BU in areas where TB is endemic. Based on these results, we are isolating and characterizing these two M. ulcerans antigens for additional testing. The N-terminal sequence for the 38/36-kDa protein has already been determined as part of the purification process for this protein, and identification and purification of the 70-kDa protein are under way. If a serologic test proves to be diagnostic, early excision of nodules and antimycobacterial chemotherapy trials of patients could reduce the public health and socioeconomic impact of this emerging disease. Acknowledgments We thank John Stanford for providing the Burulin reagent, Jennifer Ekmark for discussion and critical reading of the manuscript, Merywin Wigley for laboratory assistance, Carolyn Carter for N-terminal sequence analysis, the Emory Medical Care Foundation for collection and use of the TB patient and control sera (HIC # 455-96), and the National Center for Infectious Diseases for the initial case study of BU disease in Cote d'Ivoire. This study was supported in part by Centers for Disease Control and Prevention Cooperative agreement No. U50/CCU416560-01-1, Novel Diagnostic Tests for Infections of Public Health Significance, and by an Oak Ridge Institute for Science and Education The Oak Ridge Institute for Science and Education (ORISE) is a U.S. Department of Energy institute focusing on scientific initiatives to research health risks from occupational hazards, assess environmental cleanup, respond to radiation medical emergencies, support national Fellowship awarded to Karen M. Dobos. References (1.) Horsburgh CR Jr, Meyers WM. Buruli ulcer. In: Pathology of emerging infections. Horsburgh CR Jr, Nelson AM, editors. Washington: American Society for Mibrobiology Press; 1997. p. 11926. (2.) Dobos KM, Horsburgh CR Jr, Ashford DA, Quinn FD, King CH. Emergence of a unique group of necrotizing mycobacterial diseases. Emerg Infect Dis 1999;5:367-78. (3.) Marston BJ, Diallo MO, Horsburgh CR Jr, Diomande I, Saki MZ, Kanga Kanga may refer to: Places
(4.) Amofah GK, Sagoe-Moses C, Adjei-Acquah C, Frimpong EH. Epidemiology of Buruli ulcer in Amansie West district The Amansie West District is a district of Ghana in the Ashanti Region. Sources
(5.) Hayman J. Postulated epidemiology of Mycobacterium ulcerans infection. Int J Epidemiol 1991 ;20:1093-8. (6.) Portaels F, Elsen P, Guimaraes-Peres A, Fonteyne PA, Meyers WM. Insects in the transmission of Mycobacterium ulcerans infection. Lancet 1999;353:986. (7.) Asiedu K, Etuaful S. Socioeconomic implications of Buruli ulcer in Ghana: a three-year review. Am J Trop Med Hyg 1998;59:1015-22. (8.) Amofah G, Asamoah S, Afram-Gyening G. Effectiveness of excision of pre-ulcerative Buruli lesions in field situations in a rual district in Ghana. Trop Doct 1998;28:81-3. (9.) Stanford TL, Revill WDL WDL Windows Driver Library WDL World Definition Language (3D GameStudio programming language) WDL Winter Drumline WDL Wavelength Dependent Loss WDL Waveform Description Language , Gunthorpe WJ, Grange JM. The production and preliminary investigation of Burulin, a new skin test for Mycobacterium ulcerans infection. Journal of Hygiene (London) 1975;74:7-16. (10.) Laemmli UK. Cleavage of structural proteins during the assembly of the head of bacteriophage T4. Nature 1970;227:680-5. (11.) Morrissey JH. Silver stain for proteins in polyacrylamide gels: a modified procedure with enhanced, uniform sensitivity. Anal Biochem 1981;117:307-10. (12.) O'Farrell PH. High resolution two dimensional analysis of proteins. J Biol Chem 1975;250:4007-21. (13.) Sonnenberg MG, Belisle JT. Definition of Mycobacterium tuberculosis culture filtrate proteins by two dimensional polyacrylamide gel electrophoresis, N-terminal amino acid sequencing, and electrospray mass spectrometry. Infect Immun 1997;65:4515-24. (14.) Towbin H, Staehelin T, Gordon J. Electrophoretic transfer of protein from polyacrylamide gels to nitrocellulose nitrocellulose, nitric acid ester of cellulose (a glucose polymer). It is usually formed by the action of a mixture of nitric and sulfuric acids on purified cotton or wood pulp. sheets: procedure and some applications. Proc Natl Acad Sci U S A 1979;76:4350-4. (15.) Dobos KM, Khoo KH, Swiderek KM, Brennan PJ, Belisle JT. Definition of the full extent of glycosylation of the 45-kilodalton glycoprotein of Mycobacterium tuberculosis. J Bacteriol 1996;178:2498-506. (16.) De Vries RR. An immunogenetic view of delayed type hypersensitivity. Tubercle tubercle (t  `bərkyl') [Lat.,=little swelling], small, usually solid, nodule or prominence. 1991;72:161-7.(17.) Sengupta U. Studies on lepromin and soluble antigens of M. leprae: their classification standardization and use. Indian J Lepr 1991;63:457-65. (18.) Shield MJ, Stanford JL, Paul RC, Carswell JW. Multiple skin testing of tuberculosis patients with a range of new tuberculins, and acomparison with leprosy and Mycobacterium ulcerans infection. Journal of Hygiene (London) 1977;78:331-48. (19.) Dannenberg AM Jr. Delayed-type hypersensitivity and cell-mediated immunity in the pathogenesis of tuberculosis. Immunol Today 1991;7:228-33. (20.) Orme IM, Andersen P, Boom WH. T cell response to Mycobacterium tuberculosis. J Infect Dis 1993;167:1481-97. (21.) Belisle JT, Vissa VD, Sievert sie·vert n. Abbr. Sv A unit of ionizing radiation absorbed dose equivalent in the International System of Units, obtained as a product of the absorbed dose measure in grays and a dimensionless factor, stipulated by the International T, Takayama K, Brennan PJ, Besra GS. Role of the major antigen of Mycobacterium tuberculosis in cell wall biogenesis biogenesis /bio·gen·e·sis/ (-jen´e-sis) 1. origin of life, or of living organisms. 2. the theory that living organisms originate only from other living organisms. . Science 1997;276:1420-2. Karen M. Dobos,(*)([dagger]) Ellen A. Spotts,(*)([dagger]) Barbara J. Marston,(*) C. Robert Horsburgh Jr.,(*) and C. Harold King(*) (*) Emory University School of Medicine, Atlanta, Georgia, USA; and ([dagger]) Centers for Disease Control and Prevention, Atlanta, Georgia, USA Dr. Dobos is a senior postdoctoral fellow in the laboratory of Dr. C. Harold King at the Emory University School of Medicine. Her current research interests focus on bacterial proteomic analysis. She will continue studying the proteins of Mycobacterium ulcerans for development of future vaccine and diagnostic candidates. Address for correspondence: C. Harold King, Emory University School of Medicine, 69 Butler St. S.E., Atlanta, GA 30303, USA; fax: 404-880-9305; e-mail: cking01@emory.edu |
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