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Issa, Nicolas

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Issa

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Nicolas

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Issa, Nicolas
Author's Publications: search.filters.isAuthorOfPublication.0102268a-1e2a-4b89-ad76-8b6505a08c57

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    Green Herring Syndrome: Bacterial Infection in Patients With Mucormycosis Cavitary Lung Disease

    (Oxford University Press, 2014) Peixoto, Driele; Hammond, Sarah; Issa, Nicolas; Madan, Rachna; Gill, Ritu; Milner, Danny; Colson, Yolonda; Koo, Sophia; Baden, Lindsey; Marty, Francisco

    Mucormycosis is a life-threatening fungal disease in patients with hematological malignancies. The diagnosis of pulmonary mucormycosis is particularly challenging. We describe 3 mucormycosis cases with an uncommon presentation in patients whose cavitary lung disease was attributed to well documented bacterial infection, although evolution and reassessment established mucormycosis as the underlying disease.

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    Absence of Replication of Porcine Endogenous Retrovirus and Porcine Lymphotropic Herpesvirus Type 1 with Prolonged Pig Cell Microchimerism after Pig-to-Baboon Xenotransplantation

    (American Society for Microbiology, 2008) Issa, Nicolas; Wilkinson, R. A.; Griesemer, Adam; Cooper, David K. C.; Yamada, Kazuhiko; Sachs, David; Fishman, Jay

    Porcine endogenous retrovirus (PERV), porcine cytomegalovirus (PCMV), and porcine lymphotropic her- pesvirus (PLHV) are common porcine viruses that may be activated with immunosuppression for xenotrans- plantation. Studies of viral replication or transmission are possible due to prolonged survival of xenografts in baboon recipients from human decay-accelerating factor transgenic or -1,3-galactosyltransferase gene knock- out miniature swine. Ten baboons underwent xenotransplantation with transgenic pig organs. Graft survival was 32 to 179 days. Recipient serial samples of peripheral blood mononuclear cells (PBMC) and plasma were analyzed for PCMV, PERV, and PLHV-1 nucleic acids and viral replication using quantitative PCR assays. The PBMC contained PERV proviral DNA in 10 animals, PLHV-1 DNA in 6, and PCMV in 2. PERV RNA was not detected in any PBMC or serum samples. Plasma PLHV-1 DNA was detected in one animal. Pig cell micro- chimerism (pig major histocompatibility complex class I and pig mitochondrial cytochrome c oxidase subunit II sequences) was present in all recipients with detectable PERV or PLHV-1 (85.5%). Productive infection of PERV or PLHV-1 could not be demonstrated. The PLHV-1 viral load did not increase in serum over time, despite prolonged graft survival and pig cell microchimerism. There was no association of viral loads with the nature of exogenous immune suppression. In conclusion, PERV provirus and PLHV-1 DNA were detected in baboons following porcine xenotransplantation. Viral detection appeared to be due to persistent pig cell microchimerism. There was no evidence of productive infection in recipient baboons for up to 6 months of xenograft function.