Cell-Mediated Immune Response to Tuberculosis Antigens: Comparison of Skin Testing and Measurement of In Vitro Gamma Interferon Production in Whole-Blood Culture

doi:10.1128/CDLI.8.2.339-345.2001

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Clinical and Diagnostic Laboratory Immunology, March 2001, p. 339-345, Vol. 8, No. 2
1071-412X/01/$04.00+0 DOI: 10.1128/CDLI.8.2.339-345.2001

Cell-Mediated Immune Response to Tuberculosis Antigens: Comparison of Skin Testing and Measurement of In Vitro Gamma Interferon Production in Whole-Blood Culture

Rohit K. Katial,¹^,^* Joyce Hershey,¹ Tejashiri Purohit-Seth,¹ John T. Belisle,² Patrick J. Brennan,² John S. Spencer,² and Renata J. M. Engler¹

Allergy-Immunology Department, Walter Reed Army Medical Center, Washington, D.C.,¹ and Department of Microbiology, Colorado State University, Fort Collins, Colorado²

Received 7 August 2000/Returned for modification 19 October 2000/Accepted 8 December 2000

Although delayed-type hypersensitivity skin testing with tuberculin purified protein derivative (PPD) is the standard fortuberculosis screening, its variability suggests the need fora more sensitive, noninvasive test. An in vitro whole-blood assayhas been proposed as an alternative. Using health care workervolunteers, we confirmed the correlation between PPD skin test(PPD-ST) results (positive, induration of >15 mm) and a standardizedgamma interferon (IFN- $gamma$ ) assay, QuantiFERON-TB (Q-IFN), manufacturedby CSL Biosciences in Australia, and we evaluated Mycobacteriumtuberculosis culture subfractions as potential substitutes forPPD. Twenty healthy volunteers with positive PPD-ST results and20 PPD-ST-negative controls were enrolled. Whole blood was culturedwith human PPD antigens (HuPPD), Mycobacterium avium complex (MAC)PPD, phytohemagglutinin (PHA), and four M. tuberculosis culturesubfractions: low-molecular-weight culture, filtrate, culturefiltrate without lipoarabinomannan, soluble cell wall proteins,and cytosolic proteins, all developed from M. tuberculosis strainH₃₇RV. Secretion of IFN- $gamma$ (expressed as international units permilliliter) was measured by an enzyme immunoassay. The PPD orsubculture fraction response as a percentage of the PHA responsewas used to determine positivity. Sixteen of 20 PPD-ST-positiveindividuals were classified as M. tuberculosis positive by Q-IFN,and 1 was classified as MAC positive. Sixteen of 20 PPD-ST-negativeindividuals were M. tuberculosis negative by Q-IFN, 2 were MACpositive, and 2 were M. tuberculosis positive. The tuberculosisculture subfractions stimulated IFN- $gamma$ production in PPD-ST-positivevolunteers, and significant differences could be seen betweenthe two PPD-ST groups with all subfractions except soluble cellwall protein; however, the response was variable and no betterthan the Q-IFN PPD. The agreement between the Q-IFN test and thePPD-ST was good (Cohen's kappa = 0.73). The Q-IFN assay can bea useful tool in further studies of immune responses to M. tuberculosisantigens.

^* Corresponding author. Mailing address: Walter Reed Army Medical Center, Allergy-Immunology Clinic, 6900 Georgia Ave., Washington,DC 20307. Phone: (202) 782-8085. Fax: (202) 782-7093. E-mail:rohit.katial{at}amedd.army.mil.

Clinical and Diagnostic Laboratory Immunology, March 2001, p. 339-345, Vol. 8, No. 2
1071-412X/01/$04.00+0 DOI: 10.1128/CDLI.8.2.339-345.2001

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