, 2005). Among the positive clinical samples, 68.9% (31/45) were cutaneous biopsies, 17.8% (8/45) were cutaneous swabs, 4.4% (2/45) were total blood samples and 8.9% (4/45) were serum samples. The identification of rickettsial infections using cutaneous swab specimens and PCR testing has recently been reported (Bechah et al., 2011; Mouffok et al., 2011); based on these preliminary results, we collected cutaneous swabs from patients rather selleck screening library than cutaneous biopsies. Our retrospective analysis recovered eight positive cutaneous eschar swabs from different patients, confirming that these provide a rapid and simple means method that can be performed easily without the
risk of the side effects related to biopsy collection in patients who display an inoculation eschar and/or a vesicular rash (Mouffok et al., 2011). In conclusion, the widespread use of qPCR is less expensive than conventional PCR and reduces delay in the diagnosis of rickettsial infections. The development of qPCR strategies in the diagnosis of rickettsioses has previously Ganetespib been proposed (Stenos et al., 2005). Our 2 years of experience of rickettsial diagnosis using qPCR suggests that these molecular tools improve the efficiency of the management of patients with suspected cases of rickettsiosis. These qPCR assays could therefore
be easily implemented in laboratories with molecular facilities and may be added to existing molecular tools as a point-of-care strategy (Holland & Kiechle, 2005). “
“Semen is the primary medium for sexual transmission of HIV-1 and contains high concentrations of TGF-β1,
but its role in regulating HIV-mediated immune activation is unclear. TGF-β1 and sCD14 were compared in blood plasma (BP) and seminal plasma (SP) from HIV-uninfected and infected, antiretroviral therapy (ART)-naive and ART-treated men and in THP-1 nearly cells following exposure to HIV-1. The relationship between TGF-β1 and sCD14 was determined by Spearman correlation. Active and latent forms of TGF-β1 were compartmentalized between BP and SP. Highest active TGF-β1 levels were present in SP of ART-naïve chronic-infected men and decreased following ART treatment. Latent TGF-β1 was upregulated in BP following HIV infection, and highest levels were observed in BP of acute-infected men. Similar expression trends were observed between latent TGF-β1 and sCD14 in BP. A significant negative correlation was observed between active TGF-β1, sCD14, and semen viral load in ART-naive men. TGF-β1 is compartmentalized between blood and semen, possibly co-expressed with sCD14 by activated monocytes/macrophages in BP as a result of HIV infection. Conversion of latent TGF-β1 into its active form could contribute to regulation of viral load and immune activation in the male genital tract, but depends on the stage of infection.