HCMV infection was associated

HCMV infection was associated check details to an increase of NKG2Cbright NK cells [26] shown to display a CD57+ phenotype [32]. We originally reported that, as compared to the NKG2A+ NK-cell subset, this population contained higher proportions of LILRB1+ and KIR+ cells, but displayed lower surface levels of NKp46 and NKp30 NCR [26]. Studies in several samples confirmed this immunophenotypic pattern in children

with congenital HCMV infection (data not shown); to what extent the persistent NKR redistribution might condition the innate response to other infections and tumors deserves attention. A marked increase of LILRB1+ NK cells was also observed in symptomatic congenital HCMV infection, as compared to the other groups. The LILRB1 inhibitory receptor is expressed at late differentiation stages by cytotoxic T lymphocytes specific for different microbial pathogens [49-52]. Similarly to T lymphocytes, activated

NK cells undergo clonal expansions, experiencing differentiation events that modify their phenotype and survival [42, 53]. In this regard, LILRB1 is displayed by a variable fraction of CD56dim NK cells mTOR inhibitor [4], whereas it appears virtually undetectable in the CD56bright subset, which was shown to bear longer telomeres [54]. In the same line, most LILRB1+ cells were predominantly found among the CD27-negative cell population [4], corresponding to late NK differentiation stages [55]. Recent studies indicate that LILRB1 expression may be also upregulated in NK cells Astemizole upon in vitro

exposure to cytokines [56]. Hence, the marked increase of LILRB1+ NK populations in symptomatic congenital HCMV infection likely reflects the accumulation of cells activated/differentiated under the pressure of the pathogen. HCMV congenital symptomatic infection was also associated to higher proportions and absolute numbers of NKG2C+ and LILRB1+ T cells. Yet, the pattern was different to that observed in NK cells, as NKG2A+ and CD161+ T lymphocytes were also increased. NKR expression has been associated to late differentiation stages of TcRαβ+ CD4+ and CD8+ T cells, modulating their Ag-specific response [51, 57]. NKR may be also expressed by TcRγδ+ T cells and were detected in a subset of TcRγδ+ T cells specifically responding to congenital HCMV infection [23]. Further studies are required to more precisely define the NKR distribution in different T-cell subsets and their functional implications in congenital HCMV infection. The frequency of the NKG2C gene deletion appeared comparable in children with congenital infection and controls. Further studies in a larger cohort are required to address whether the NKG2C genotype might have a more subtle influence on the pathogenesis and/or clinical outcome of congenital HCMV infection. Remarkably, HCMV-infected NKG2C+/+ children exhibited greater numbers of circulating NKG2C+ cells than heterozygous individuals.

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