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IP-10 is an additional marker to evaluate the RD1-specific responses in HIV-infected subjects

Valentina Vanini, Teresa Chiacchio, Cristiana Gioia, Gilda Cuzzi, Nicoletta Orchi, Alessia Rianda, Lucia Alba, Maria Letizia Giancola, Aristide Conte, Elisa Petruccioli, Linda Petrone, Enrico Girardi, Delia Goletti
European Respiratory Journal 2011 38: p4386; DOI:
Valentina Vanini
1Epidemiology and Preclinical Research, INMI, Rome, Italy
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Teresa Chiacchio
1Epidemiology and Preclinical Research, INMI, Rome, Italy
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Cristiana Gioia
1Epidemiology and Preclinical Research, INMI, Rome, Italy
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Gilda Cuzzi
1Epidemiology and Preclinical Research, INMI, Rome, Italy
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Nicoletta Orchi
1Epidemiology and Preclinical Research, INMI, Rome, Italy
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Alessia Rianda
2Clinical Department, INMI, Rome, Italy
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Lucia Alba
2Clinical Department, INMI, Rome, Italy
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Maria Letizia Giancola
2Clinical Department, INMI, Rome, Italy
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Aristide Conte
2Clinical Department, INMI, Rome, Italy
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Elisa Petruccioli
1Epidemiology and Preclinical Research, INMI, Rome, Italy
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Linda Petrone
1Epidemiology and Preclinical Research, INMI, Rome, Italy
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Enrico Girardi
1Epidemiology and Preclinical Research, INMI, Rome, Italy
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Delia Goletti
1Epidemiology and Preclinical Research, INMI, Rome, Italy
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Abstract

Background: The suboptimal sensitivity of IFN-γ-based assays, especially in immunocompromised individuals, emphasizes the need for alternative markers for diagnosing tuberculosis (TB). Objective of this study was to evaluate whether IP-10 can be a useful biomarker for evaluating a specific response to RD1 antigens associated to active TB in HIV-infected individuals. Control with QuantiFERON-TB Gold In tube (QFT-IT) was performed.

Methodology: 118 HIV-infected individuals were prospectively enrolled in Rome, 21 with active-TB and 98 without. Epidemiological characteristics were analyzed. IFN-γ and IP-10 response to QFT-IT was performed. Plasma was harvested at day-1 and soluble factors evaluated by ELISA.

Results: Significant differences between those with or without active TB were found for the CD4+ T cell counts (p=0.02), and IFN-γ and IP-10 response to QFT-IT (p=0.001 for both analysis). Differently no significant differences were found for the age and HIV-RNA. Based on the commercial cut-off of the QFT-IT and on a cut-off found by ROC analysis for the IP-10-based responses, the sensitivity for active TB of QFT-IT and the IP-10 to QFT-IT was 52% and 67% respectively (p=0.001; K: 0.545). The response to IP-10 was not influenced by the ability to respond to the mitogen. The specificity for active TB of QFT-IT and of the experimental test were 84% and 77% respectively (p=0.01; k:0.710). Among those without active TB a significant correlation between a positive score and Mtb exposure was found (p<0.001).

Conclusions: These data suggest that IP-10 is an additional marker to evaluate the RD1-specific responses in HIV-subjects confirming data previously obtained in high TB endemic countries.

  • © 2011 ERS
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IP-10 is an additional marker to evaluate the RD1-specific responses in HIV-infected subjects
Valentina Vanini, Teresa Chiacchio, Cristiana Gioia, Gilda Cuzzi, Nicoletta Orchi, Alessia Rianda, Lucia Alba, Maria Letizia Giancola, Aristide Conte, Elisa Petruccioli, Linda Petrone, Enrico Girardi, Delia Goletti
European Respiratory Journal Sep 2011, 38 (Suppl 55) p4386;

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IP-10 is an additional marker to evaluate the RD1-specific responses in HIV-infected subjects
Valentina Vanini, Teresa Chiacchio, Cristiana Gioia, Gilda Cuzzi, Nicoletta Orchi, Alessia Rianda, Lucia Alba, Maria Letizia Giancola, Aristide Conte, Elisa Petruccioli, Linda Petrone, Enrico Girardi, Delia Goletti
European Respiratory Journal Sep 2011, 38 (Suppl 55) p4386;
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