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253


Comparison of PCR and standard cytological staining for detection of Pneumocystis carinii from respiratory specimens from patients with or at high risk for infection by human immunodeficiency virus [published erratum appears in J Clin Microbiol 1996 Jan;34(1):236]

Leibovitz E; Pollack H; Moore T; Papellas J; Gallo L; Krasinski K; Borkowsky W
The detection of Pneumocystis carinii DNA by PCR was compared with routine cytologic staining techniques (CYT). A total of 284 clinical respiratory specimens, including 137 bronchoalveolar lavage (BAL), 63 bronchoalveolar washing, 63 sputum, and 21 induced sputum samples, obtained from patients with or at high risk for human immunodeficiency virus infection were evaluated. Eighty specimens were positive by PCR, and 69 were positive by CYT. PCR was able to detect P. carinii in more bronchoalveolar washing specimens (15 versus 11) and in comparable BAL specimens (53 versus 54) compared with CYT. PCR was particularly more sensitive than CYT in detecting P. carinii in expectorated sputum (12 versus 4 samples). Of the 19 patients whose respiratory specimens were positive for P. carinii by PCR but negative by CYT, 5 had P. carinii pneumonia (PCP) confirmed by subsequent BAL and transbronchial or mediastinal lymph node biopsy and 9 had a clinical course highly suggestive of acute PCP. Eleven (58%) of the 19 patients with discordant PCR and CYT results had received prior anti-PCP prophylaxis. In this clinical setting in particular and in the evaluation of sputum specimens, the ability of PCR to detect a low parasitic load suggests that this technique may become an important additional tool, along with current cytological methods, for the detection of P. carinii
PMCID:228623
PMID: 8576362
ISSN: 0095-1137
CID: 7195

Shortened survival in infants vertically infected with human immunodeficiency virus with elevated p24 antigenemia

Arlievsky NZ; Pollack H; Rigaud M; Kaul A; Krasinski K; Borkowsky W
OBJECTIVE: To determine whether the amount of p24 antigenemia in the first 6 months of life is a predictor of survival in children infected vertically with human immunodeficiency virus type 1. METHODS: A retrospective study of vertically infected infants and children who were followed prospectively from early infancy and who had quantitation of plasma p24 antigen concentration in the first 6 months of life. Infants were first stratified by duration of survival as infants who died before 2 years of age (short-term survivors) and infants who survived to 2 years of age (intermediate-term survivors). The median p24 antigen concentration and the proportion of infants in each group with high concentrations of antigen were compared. Analyses with and excluding all p24 determinations made after the use of antiretroviral agents were compared Kaplan-Meier product limit analysis was used to compare survival in infants with low and high antigenemia during the first 6 months of life. RESULTS: The median p24 antigen concentration in 15 short-term survivors was 228 pg/ml, compared with 14 pg/ml in 26 intermediate-term survivors (p < 0.05). The proportion of children with > 100 pg/ml of p24 was higher in short-term than in intermediate-term survivors (p = 0.01). Survival to 2 years of age in infants in whom all p24 antigen values during the first 6 months of life were 100 pg/ml or less was 91%, in comparison with 39% in infants with values greater than 100 pg/ml (p = 0.0017). CONCLUSIONS: Elevated p24 antigenemia in the first 6 months of life is associated with shorter survival and may be a useful predictor of outcome
PMID: 7562273
ISSN: 0022-3476
CID: 6802

The sensitivity of HIV-1 DNA polymerase chain reaction in the neonatal period and the relative contributions of intra-uterine and intra-partum transmission [see comments] [Comment]

Dunn DT; Brandt CD; Krivine A; Cassol SA; Roques P; Borkowsky W; De Rossi A; Denamur E; Ehrnst A; Loveday C
OBJECTIVE: To derive reliable estimates of the sensitivity of HIV-1 DNA polymerase chain reaction (PCR) in the neonatal period and to quantify the relative contributions of intra-uterine and intra-partum transmission. METHODS: After reviewing studies on the early diagnosis of HIV-1 infection, investigators were asked to provide published and unpublished PCR test results on prospectively followed, non-breastfed, vertically infected children. Age-specific estimates of the sensitivity of PCR were derived using distribution-free methods for interval-censored data. RESULTS: Data on 271 infected children were combined for analysis. PCR detected HIV-1 DNA in an estimated 38% [90% confidence interval (CI), 29-46] of HIV-infected children tested on the day of, or day after, birth. Sensitivity was observed to rise rapidly in the second week of life, reaching 93% (90% CI, 76-97) by 14 days of age. CONCLUSION: The sensitivity of PCR in the neonatal period is higher than previously reported. This affects the clinical interpretation of an early negative test result and encourages the use of PCR as an endpoint for trials to evaluate interventions to reduce vertical transmission in non-breastfed populations. Approximately one-third of vertically acquired HIV-1 infection could be attributable to intra-uterine transmission
PMID: 8527070
ISSN: 0269-9370
CID: 14558

Polymerase chain reaction is more sensitive than standard cytologic stains in detecting Pneumocystis carinii in bronchoalveolar lavages from human immunodeficiency virus type 1-infected infants and children with pneumonia

Leibovitz E; Pollack H; Rigaud M; Kaul A; Persaud D; Gallo L; Papellas J; Krasinski K; Borkowsky W
PMID: 8532434
ISSN: 0891-3668
CID: 7910

Protective effect of interferon-alpha against cell-mediated human immunodeficiency virus transmission resulting from coculture of infected lymphocytes with fetal trophoblasts

Bourinbaiar AS; Krasinski K; Borkowsky W; Lee-Huang S
The hypothesis that the low transmission rate of HIV in utero may be due, in part, to the protective effect of IFN-producing placental trophoblasts was explored in vitro. The model consisted of H9 lymphocytes, as surrogates of maternal HIV-infected T cells, incubated for 3 h with JEG-3 trophoblasts in the presence of 10-fold dilutions of leukocyte-derived IFN-alpha (from 1000 to 0.1 IU/ml). The dose effect was monitored either directly, by measuring the levels of proviral DNA by PCR after a single round of infection, or indirectly, by coculturing infected JEG-3 with cord blood-derived MT-4 lymphocytes and determining the levels of p24 production by ELISA. Both assays revealed a dose-dependent blocking effect of IFN-alpha on cell-mediated HIV transmission. The complete inhibition of HIV infection was observed in the presence of 100 IU IFN-alpha. The efficacy of such a low dose could not be attributed to insufficient viral load because up to 10(8) infectious particles could be transmitted during cell-cell contact. An adhesion assay ruled out the possibility that IFN-alpha acts through prevention of lymphocyte-trophoblast contact. The results suggest that physiologic levels of IFN-alpha, present in the placental environment, may contribute to the protection of the fetus against HIV infection
PMID: 7553219
ISSN: 1079-9907
CID: 6582

Acute renal failure in a human immunodeficiency virus-infected child secondary to bilateral fungus ball formation [Case Report]

Papaevangelou V; Lawrence R; Kaul A; Lefluer R; Ambrosino M; Krasinski K; Borkowsky W
PMID: 7638023
ISSN: 0891-3668
CID: 6856

CORRELATION BETWEEN THE MAGNITUDE OF VIRAL LOAD IN EARLY INFANCY AND SURVIVAL AMONG PERINATALLY HIV-INFECTED CHILDREN [Meeting Abstract]

POLLACK, H; ARLIEVSKY, N; RIGAUD, M; KAUL, A; KRASINSKI, K; BORKOWSKY, W
ISI:A1995QT86500833
ISSN: 0730-2312
CID: 87326

Production of a human anti-CD4 monoclonal antibody with antiidiotype to anti-HIV type 1 glycoprotein 120

Karpatkin S; Nardi MA; Liu LX; Kouri YH; Borkowsky W
Human anti-CD4 IgG antibodies from 3 HIV-1-infected patients were affinity purified and shown to inhibit HIV-1 binding and infection of HBP-T cells. Lymphocytes from patient A, whose anti-CD4 inhibited HIV-1 binding by 68% and infection by 72%, were cultured and transformed with EBV. A human monoclonal antiidiotype antibody against anti-HIV-1 gp120 (2B) was produced, which inhibited infection of HBP-T cells by 68% at 1 microgram/ml. Mice were immunized with 2B to determine whether this anti-CD4 could be an internal image antiidiotype against anti-HIV-1 gp 120 (Ab1). Two mice produced antisera reactive with rgp120 on ELISA, whereas immunization with normal IgG produced minimal reactivity compared to unreactive normal mouse sera. However, immunoblot competition studies in which affinity-purified anti-HIV-1 gp120 (Ab1) bound to the gp120 band on nitrocellulose strips in the presence of 2B demonstrated enhancement of signal (i.e., binding of Ab2 to Ab1), rather than inhibition of Ab1 binding. Thus 2B is not an internal image of the paratope of anti-HIV-1 gp120 but yet it is capable of inducing an antibody against rgp120. This indicates that the anti-CD4 (Ab2) does bind to the binding site of Ab1, but not as a complete internal image. These data indicate the production of a human monoclonal antiidiotype antibody that inhibits binding of HIV-1 to CD4 and induces the production of antibody against HIV-1 gp120, without being an internal image antiidiotype (Ab2 beta)
PMID: 7632465
ISSN: 0889-2229
CID: 6656

Subacute pneumococcal pericarditis in a patient who did not develop tamponade [Letter]

Arlievsky N; Rigaud M; Pollack H; Borkowsky W; Krasinski K
PMID: 7888557
ISSN: 1058-4838
CID: 14559

HIV-1 infected children with severe immunodeficiency: survival and prognostic factors [Meeting Abstract]

Papaevangelou V; Pollack H; Kaul A; Lawrence R; Krasinski K; Borkowsky W
Objective: To study the survival and identify prognostic laboratory indicators for HIV-1 infected children with severe immunodeficiency (CD4 less than 15%). Methods: Kaplan-Meier product-limit analysis, from the time of severe immunodeficiency (i.e. presentation with CD4 less than 15% or persistent levels of CD4 less than 15%), was performed on HIV-1 infected children. Plasma p24 antigen and serial hemoglobin concentrations were reviewed as possible prognostic indicators of survival. Results: (Table: see text.) The presence of plasma p24 antigen at presentation did not appear to affect survival in children with CD4 between 10-15%, however the absence of detectable plasma p24 antigen was associated with increased survival in those with CD4 of less than 10% at presentation (50% survival 4.5y and 3.4y for children with CD4 5-9% and 0-4% respectively). A 15% reduction in serum hemoglobin concentration, was associated with decreased 50% survival only in children with CD4 less than 10% (6.2y vs 2.3y). Conclusions: Children with 9 greater than CD4% less than 15% are considered to be severely immunodeficient by the CDC, yet their 50% survival is significantly better than children who present with CD4 less than 10%. The absence of detectable p24 antigenemia at presentation appeared to be associated with improved survival only in children with CD4 T cells less than 10%, whereas a 15% decrease in serum hemoglobin concentration was associated with lower survival only in those with greater than 10% CD4 T cells
BCI:BCI199598024920
ISSN: 1532-0227
CID: 5994