Potential Serological Use of a Recombinant Protein That Is a Replica of aMycobacterium tuberculosisProtein Found in the Urine of Infected Mice | Zendy

Sandeep Mukherjee | Zendy; Nada Daifalla | Zendy; Yanni Zhang | Zendy; John F. Douglass | Zendy; Lisa Brooks | Zendy; Thomas Vedvick | Zendy; Raymond L. Houghton | Zendy; Steven G. Reed | Zendy; Antonio CamposNeto | Zendy

Open Access

Potential Serological Use of a Recombinant Protein That Is a Replica of aMycobacterium tuberculosisProtein Found in the Urine of Infected Mice

Author(s) -

Sandeep Mukherjee,

Nada Daifalla,

Yanni Zhang,

John F. Douglass,

Lisa Brooks,

Thomas Vedvick,

Raymond L. Houghton,

Steven G. Reed,

Antonio CamposNeto

Publication year - 2004

Publication title -

clinical and vaccine immunology

Language(s) - English

Resource type - Journals

SCImago Journal Rank - 1.649

H-Index - 77

eISSN - 1556-6811

pISSN - 1556-679X

DOI - 10.1128/cdli.11.2.280-286.2004

Subject(s) - mycobacterium tuberculosis , tuberculosis , serology , antigen , virology , recombinant dna , coinfection , antibody , biology , immunology , medicine , virus , pathology , gene , biochemistry

The recent availability of numerous well-characterized Mycobacterium tuberculosis recombinant proteins has revived interest in the serological diagnosis of tuberculosis. Several promising results have been reported, particularly when more than one antigen is used in the test. However, thus far these antigens have not been used in routine diagnostic tests because they lack sufficient sensitivity. In addition, with the exception of one antigen, most recombinant M. tuberculosis proteins do not identify the majority of tuberculosis patients coinfected with human immunodeficiency virus (HIV). Here, we report a newer M. tuberculosis protein that is a promising candidate for increasing the sensitivity of the serological tests, in particular for patients coinfected with HIV. The protein was found in the urine of mice during the early stages of infection with M. tuberculosis (10 to 14 days), thus suggesting that the antigen is abundantly released during the in vivo growth of the mycobacterium. Reverse genetics was used to produce the recombinant protein, which we named U1 (for urine protein 1). Using a conventional enzyme-linked immunosorbent assay (ELISA), antibody to U1 could be detected in 60% of patients with pulmonary tuberculosis with no signs of coinfection with HIV (n = 83). Conversely, anti-U1 antibody was detected in 87% of the sera from tuberculosis patients coinfected with HIV (n = 47). Out of 12 HIV-infected nontuberculosis patients' sera, 9 did not react with U1 and three sera gave borderline ELISA signals (signal/cutoff of < or =1.75). These results suggest that the high efficiency of U1 in identifying tuberculosis patients coinfected with HIV may be related to abundant release of this protein during the initial phase of the HIV coinfection. The immediate availability of the antigen at a time point in which the patient's immune system is still competent would lead to a secondary immune response to U1 that persists for months in the patient's serum.

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