Inorganic Supramolecular Host Architectures:  [(M@18c6)2][TlI4]·2H2O, M = 0.5 Tl, (NH4,NH3), (H3O,H2O)

Administration of IL-2 to HIV-infected patients leads to expansion of a unique subset of CD4 + CD45RO -CD25 + cells. In this study, the origin, clonality, and function of these cells were investigated. Analysis of TCR excision circles revealed that the CD4 + CD45RO -CD25 + cells were the product of peripheral expansion but remained polyclonal as determined by TCR repertoire analysis. Phenotypically, these cells were distinct from naturally occurring Tregs; they exhibited intermediate features, between those of memory and naive cells, and had lower susceptibility to apoptosis than CD45RO -CD25 -or memory T cells. Studies of intracellular cytokine production and proliferation revealed that cytokine-expanded naive CD25 + cells had low IL-2 production and required costimulation for proliferation. Despite elevated expression of forkhead transcription factor P3 (foxP3), they exerted only weak suppression compared with CD45RO + CD25 +high cells (Tregs). In summary, in vivo IL-2 administration to HIV-infected patients leads to peripheral expansion of a population of longlived CD4 + CD45RO -CD25 + cells that express high levels of foxP3 but exert weak suppressive function. These CD4 + CD25 + cytokine-expanded naive cells, distinct from antigen-triggered cells and Tregs, play a role in the maintenance of a state of low turnover and sustained expansion of the CD4 + T cell pool.

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Estimation of nasal epithelial lining fluid using urea as a marker

Kaulbach¹,

White²,

Igarashi³

et al. 1993

Journal of Allergy and Clinical Immunology

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Nasal Secretion of the Ozone Scavenger Uric Acid

Peden

Swiersz²,

Ohkubo³

et al. 1993

Am Rev Respir Dis

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Uric acid, an important scavenger of ozone, has been identified as the major low molecular weight antioxidant in baseline and cholinergically induced nasal secretions. The purpose of this study was to determine the specific tissue source of uric acid in airway secretions. The secretion of uric acid is increased by cholinergic stimulation and correlates closely with the secretion of lactoferrin (a nasal glandular protein), suggesting that submucosal glands are involved. Indeed, nasal turbinate tissue was found to contain uric acid. However, careful analysis of nasal turbinate tissue failed to reveal the presence of xanthine oxidase, the enzyme responsible for uric acid synthesis. These data suggest that uric acid might be taken up secondarily by glands from plasma. This possibility was strengthened by the observation that lowering the plasma urate level with probenecid concomitantly lowered urate secretion. These findings are consistent with the hypotheses that the principal source of uric acid in nasal secretions is plasma and that uric acid is taken up, concentrated, and secreted by nasal glands.

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The Use of Oral Washes to DiagnosePneumocystis cariniiPneumonia: A Blinded Prospective Study Using a Polymerase Chain Reaction–Based Detection System

et al. 2001

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Pneumocystis carinii pneumonia (PCP) can be diagnosed by direct microscopic examination of induced sputum or by bronchoalveolar lavage (BAL). However, many institutions have little diagnostic success with induced sputum, and BAL is invasive and expensive. This prospective, blinded study assessed oral washes as a more convenient specimen than either sputum or BAL fluid and used a dissociation-enhanced lanthanide fluoroimmunoassay time-resolved fluorescent hybridization polymerase chain reaction (PCR) detection system that is feasible for clinical laboratories. The study assessed 175 oral washes, each paired with either an induced sputum that was positive for Pneumocystis or a BAL sample. The PCR test based on the Pneumocystis major surface glycoprotein primers had a sensitivity of 91% and a specificity of 94%, compared with a test based on mitochondrial large subunit rRNA primers, which had a sensitivity of 75% and a specificity of 96%. These results suggest that oral washes can provide a useful sample for diagnosis of PCP when a sensitive PCR detection system is used.

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Fluorodeoxyglucose imaging in healthy subjects with HIV infection: impact of disease stage and therapy on pattern of nodal activation

Brust

Polis

Davey

et al. 2006

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Barbara Hahn

In vivo expansion of CD4+CD45RO-CD25+ T cells expressing foxP3 in IL-2-treated HIV-infected patients

Estimation of nasal epithelial lining fluid using urea as a marker

Nasal Secretion of the Ozone Scavenger Uric Acid

The Use of Oral Washes to DiagnosePneumocystis cariniiPneumonia: A Blinded Prospective Study Using a Polymerase Chain Reaction–Based Detection System

Fluorodeoxyglucose imaging in healthy subjects with HIV infection: impact of disease stage and therapy on pattern of nodal activation

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