Specific, Sensitive, and Quantitative Enzyme-Linked Immunosorbent Assay for Human Immunoglobulin G Antibodies to Anthrax Toxin Protective Antigen

Quinn, Conrad P.; Semenova, Vera; Elie, Cheryl M.; Romero-Steiner, Sandra; Greene, Carolyn M.; Li, Han; Stamey, Karen; Steward‐Clark, Evelene; Schmidt, Daniel S.; Mothershed, Elizabeth A.; Pruckler, Janet M.; Schwartz, Stephanie; Benson, Robert F.; Helsel, Leta O.; Holder, Patricia; Johnson, Scott E.; Kellum, Molly; Messmer, Trudy O.; Thacker, W L; Besser, Lilah M.; Plikaytis, Brian D.; Taylor, Thomas H.; Freeman, Alison; Wallace, Kelly J.; Dull, Peter; Sejvar, Jim; Bruce, Erica D.; Moreno, Rosa L.; Schuchat, Anne; Lingappa, Jairam R.; Martin, Sandra; Walls, John; Bronsdon, Melinda A.; Carlone, George M.; Bajani-Ari, Mary; Ashford, David A.; Stephens, David S.; Perkins, Bradley A.

doi:10.3201/eid0810.020380

Cited by 194 publications

(168 citation statements)

References 27 publications

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“…A serum concentration of IgG to PA ≥ 3 g/mL was observed in all subjects after vaccination. This level of antibody, which represents the lower limit of quantification for undiluted serum using an ELISA analogous to that applied in this study [9], was reached by 39.5% of subjects after the first injection, by a total of 96.5% after the second injection, and by 100% after the third injection ( Table 4). The mean number of days after the first vaccine dose needed to reach 3 g/mL was 24.2 (range = 13-63 days).…”

Section: Igg To Pamentioning

confidence: 63%

“…Optical density (OD) values were read within 30 min by using a Bio-Tek ELx808 plate with 405 and 490 nm filters, and KC4 software (Bio-Tek Instruments, Inc., Winooski, VT). OD values were converted to immunoglobulin concentration ( g/mL) by using a standard curve calibration factor [9]. Titers were calculated as the reciprocal of the highest dilution of the test serum yielding a mean OD value ≥ the cut-off value for the assay.…”

Section: Laboratory Studiesmentioning

confidence: 99%

See 1 more Smart Citation

Patterns of antibody response in humans to the anthrax vaccine adsorbed (AVA) primary (six-dose) series☆

Pittman

Norris

Oro

et al. 2006

Vaccine

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Section: Igg To Pamentioning

confidence: 63%

Section: Laboratory Studiesmentioning

confidence: 99%

Patterns of antibody response in humans to the anthrax vaccine adsorbed (AVA) primary (six-dose) series☆

Pittman

Norris

Oro

et al. 2006

Vaccine

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“…Serology and reverse transcription (RT)-PCR were performed by other laboratories at CDC. [42][43][44] § Contained a small, superficial, shave biopsy that was inadequate for pathologic evaluation.…”

Section: Methodsmentioning

confidence: 99%

The Critical Role of Pathology in the Investigation of Bioterrorism-Related Cutaneous Anthrax

Shieh

Guarner

Paddock

et al. 2003

The American Journal of Pathology

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Cutaneous anthrax is a rare zoonotic disease in the United States. The clinical diagnosis traditionally has been established by conventional microbiological methods, such as culture and gram staining. However, these methods often yield negative results when patients have received antibiotics. During the bioterrorism event of 2001, we applied two novel immunohistochemical assays that can detect Bacillus anthracis antigens in skin biopsy samples even after prolonged antibiotic treatment. These assays provided a highly sensitive and specific method for the diagnosis of cutaneous anthrax, and were critical in the early and rapid diagnosis of 8 of 11 cases of cutaneous anthrax during the outbreak investigation. Skin biopsies were obtained from 10 of these 11 cases, and histopathological findings included various degrees of ulceration, hemorrhage, edema, coagulative necrosis, perivascular inflammation, and vasculitis. Serology was also an important investigation tool, but the results required several weeks because of the need to test paired serum specimens. Other tests, including culture, special stains, and polymerase chain reaction assay, were less valuable in the diagnosis and epidemiological investigation of these cutaneous anthrax cases. This report underscores the critical role of pathology in investigating potential bioterrorism events and in guiding epidemiological studies, Anthrax captured worldwide attention and aroused serious public health concerns following the intentional release of the etiological agent Bacillus anthracis in the United States postal system during Fall 2001, 1,2 resulting in 11 cases of inhalational anthrax and 11 cases of cutaneous anthrax. [3][4][5][6][7] In its conventional form, cutaneous anthrax accounts for 95% of all naturally occurring B. anthracis infections in the United States. 8 -11 Patients often have a history of occupational contact with animals or animal products contaminated with B. anthracis spores. 12-14 These pathogenic spores are introduced through a cutaneous cut or abrasion, with the most common areas of exposure are the head, neck, and extremities, although any area can be involved. Bacteremia and toxemia following cutaneous infection can occur with a fatality rate of 20% to 25% among untreated cases. [15][16][17] Cutaneous anthrax is characterized by the formation of a black eschar surrounded by prominent edema and vesicles, which may resemble many other skin lesions, such as the brown recluse spider bite, 18 -21 ulceroglandular tularemia, 22,23 plague, 24,25 ecthyma gangrenosum, 26,27 various spotted fever group rickettsial infections, 28 -31 and scrub typhus. 32,33 The clinical diagnosis of cutaneous anthrax is traditionally established by microbiological methods (eg, demonstrating gram-positive, capsulated bacilli on the smear of the lesion or isolating B. anthracis in culture). 34,35 However, gram stain and culture for B. anthracis can be unrevealing for patients who receive antibiotic therapy before specimens are obtained. 36,37 Historically, skin biopsies ...

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“…for standard reference serum AVR801 was used to determine the concentration of anti-PA IgG in lg/mL of test serum; the lower limit of quantification of the anti-PA ELISA was 3.7 mg/mL anti-PA IgG in undiluted serum samples; diagnostic sensitivity was 98.6% and diagnostic specificity was 98.4% (Quinn et al 2002(Quinn et al , 2004Semenova et al 2004) Anti-PA IgG concentration ‡ to the assay lower limit of quantification (3.7 lg/mL)…”

Section: Study Populationmentioning

confidence: 99%

“…Pathogens tested and specific methods of serologic testing for each of the agents evaluated have been described elsewhere (Table 1; Lindsey et al 1976;Dikken and Kmety 1978;Brown et al 1981;Dalton et al 1995;Plikaytis et al 1996;Nicholson et al 1997;Johnson et al 2000Johnson et al , 2005Martin et al 2000;Quinn et al 2002Quinn et al , 2004Dumler 2004;Semenova et al 2004;Jones et al 2007). Baseline seropositivity was interpreted as prior infection.…”

Section: Serological Testingmentioning

confidence: 99%

Zoonotic Infections Among Employees from Great Smoky Mountains and Rocky Mountain National Parks, 2008–2009

Adjemian

Weber

McQuiston

et al. 2012

Vector-Borne and Zoonotic Diseases

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Specific, Sensitive, and Quantitative Enzyme-Linked Immunosorbent Assay for Human Immunoglobulin G Antibodies to Anthrax Toxin Protective Antigen

Cited by 194 publications

References 27 publications

Patterns of antibody response in humans to the anthrax vaccine adsorbed (AVA) primary (six-dose) series☆

Patterns of antibody response in humans to the anthrax vaccine adsorbed (AVA) primary (six-dose) series☆

The Critical Role of Pathology in the Investigation of Bioterrorism-Related Cutaneous Anthrax

Zoonotic Infections Among Employees from Great Smoky Mountains and Rocky Mountain National Parks, 2008–2009

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