G.L. Rosner scite author profile

G.L. Rosner

4Publications

84Citation Statements Received

41Citation Statements Given

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187

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University of Pittsburgh, Cleveland Clinic, University of Pittsburgh Medical Center

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Large‐scale oligonucleotide typing for HLA‐DRB1/3/4 and HLA‐DQB1 is highly accurate, specific, and reliable

Hurley

Baxter‐Lowe

et al. 1993

Tissue Antigens

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DNA typing of HLA class II alleles of the DRB1/3/4 and DQB1 loci using sequence-specific oligonucleotide probes and polymerase chain reaction-amplified DNA was used for the large-scale typing of donors for the National Marrow Donor Program unrelated donor registry. The results of quality control analysis for the first 7 months of the project show the typing to be highly accurate, specific, and reliable. The percent of correctly classified HLA oligotypes based on 1652 DRB1 and 1652 DQB1 assignments was greater than 99% for DRB1/DRB3/DRB4 and greater than 98% for DQB1. This level of accuracy is particularly remarkable because the quality control samples could not be distinguished from 9011 donor samples tested at the same time by the laboratories.

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Combined Simultaneous Kidney/Bone Marrow Transplantation1

et al. 1995

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On the basis of observations in patients with long-term (28-30 years) renal allograft survival, all of whom had evidence of systemic microchimerism, we began a program of combined simultaneous kidney/bone marrow transplantation. Between 12/14/92, and 10/31/94, 36 kidney transplant recipients received 3-5 x 10(8) unmodified bone marrow cells/kg; 6 patients also received pancreatic islets, and 7 patients also received a pancreas. The mean recipient age was 39.0 +/- 10.8 years, and the mean donor age was 31.8 +/- 16.1 years; the mean cold ischemia time was 23.0 +/- 9.1 hr. Twenty control patients received kidneys alone, mainly because of refusal by the donor family to consent to vertebral body recovery; 3 of these patients also received a pancreas. The mean recipient age was 47.9 +/- 11.7 years, and the mean donor age was 41.5 +/- 17.9 years; the mean cold ischemia time was 28.6 +/- 6.2 hr. All patients received tacrolimus-based therapy, without radiation, cytoreduction, or induction antilymphocyte preparations. Blood was drawn prior to and at regular intervals after transplantation for detection of chimerism and for immunologic studies. With a mean follow-up of 11.1 +/- 5.8 months, all 36 study patients are alive, and 33 (92%) have functioning allografts with a mean serum creatinine of 1.9 +/- 1.2 mg/dl and a BUN of 26 +/- 9 mg/dl. Graft vs. host disease was not seen in any patient. The incidence of rejection was 72%; 11% of the patients required OKT3 or ATG for steroid-resistant rejection. The incidence of CMV was 14%, and that of delayed graft function was 17%. A total of 18 (90%) control patients are alive, and 17 (85%) have functioning allografts, with a mean serum creatinine of 2.1 +/- 1.3 mg/dl, and a BUN of 30 +/- 13 mg/dl. The incidence of rejection was 60%, and 10% required OKT3 or ATG. CMV was seen in 15%, and delayed graft function in 20% (P = NS). In the study patients, chimerism was detected in the peripheral blood of 30 of 31 (97%) evaluable patients by either PCR or flow cytometry. In the control patients, chimerism was seen in 9 of 14 (64%) evaluable patients (P < .02). Decreasing donor-specific responsiveness was seen in 6/29 (21%) evaluable study, and 4/14 (29%) evaluable control patients (P = NS). We conclude that combined kidney/bone marrow transplantation is associated with acceptable patient and graft survival, augmentation of chimerism, and no change in the early events after transplantation.

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cDNA cloning of human myeloperoxidase: decrease in myeloperoxidase mRNA upon induction of HL-60 cells.

Weil¹,

Rosner²,

Reid³

et al. 1987

Proc. Natl. Acad. Sci. U.S.A.

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Myeloperoxidase (MPO), the most abundant neutrophil protein, is a bacteriocidal component of the primary granules and a critical marker in distinguishing acute myelogenous leukemia from acute lymphoid leukemia. A cDNA clone for human MPO was isolated by immunologic screening of human hematopoietic Xgtll expression vector libraries with specific anti-MPO antibody. The identity of the cDNA clone was confirmed by rinding that (i) epitope-selected antibody against this clone recognizes purified MPO and MPO in human promyelocytic (HL-60) cell lysates by immunoblot analysis, and that (ii) hybrid selection of HL-60 mRNA with this cDNA clone and translation in vitro results in the synthesis of an 80-kDa protein recognized by the anti-MPO antiserum. RNA blot analysis with this MPO cDNA clone detects hybridization to two polyadenylylated transcripts of :3.6 and r2.9 kilobases in HL-60 cells. No hybridization is detected to human placenta mRNA. Upon induction of HL-60 cells to differentiate by incubation for 4 days with dimethyl sulfoxide, a drastic decrease in the hybridization intensity of these two bands is seen. This is consistent with previous data suggesting a decrease in MPO synthesis upon such induction of these cells. The MPO cDNA should be useful for further molecular and genetic characterization of MPO and its expression and biosynthesis in normal and leukemic granulocytic differentiation.Myeloperoxidase (MPO), a critical microbicidal protein of mature polymorphonuclear neutrophils, is a hemoprotein composing 3-5% of the protein weight of these cells (1, 2). It appears in the primary azurophilic granules during the differentiation of the neutrophil (3, 4) and has been used as a marker for these granules (5). Cytochemical staining of MPO activity is used clinically to distinguish acute myeloid leukemia from acute lymphoid leukemia (6). Furthermore, approximately 1 in every 2000 individuals has been shown to be deficient in MPO (7), an apparently benign but poorly understood hereditary disorder of polymorphonuclear neutrophils.Although the function of MPO in the oxygen-dependent respiratory burst of polymorphonuclear neutrophils has been firmly established, relatively little is known about MPO biosynthesis, posttranslational modification, and genetic organization and expression. The exact structure of MPO remains a source of some controversy, and its amino acid sequence is not known.The appearance of MPO in the primary granules marks the transition from the myeloblast to the promyelocyte in the course of normal neutrophilic differentiation (3). Promyelocytes, however, are not found in the peripheral blood of normal individuals and are therefore difficult to study biochemically. The HL-60 cell line, derived from a patient with acute promyelocytic leukemia, contains virtually 100%o promyelocytes with azurophilic granules containing MPO (8).When HL-60 cells are cultured in the presence of compounds such as dimethyl sulfoxide (Me2SO) (8) or retinoic acid (9), these cells mature into metamyelocytes, neutrophili...

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Perioperative donor bone marrow infusion augments chimerism in heart and lung transplant recipients

Pham

Rao

Fontes

et al. 1995

The Annals of Thoracic Surgery

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Background-We and others have demonstrated that a low level of donor cell chimerism was present for years after transplantation in tissues and peripheral blood of heart and lung recipients; it was associated, in the latter, with a lower incidence of chronic rejection. To augment this phenomenon, we initiated a trial combining simultaneous infusion of donor bone marrow with heart or lung allotransplantation.

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G.L. Rosner

Large‐scale oligonucleotide typing for HLA‐DRB1/3/4 and HLA‐DQB1 is highly accurate, specific, and reliable

Combined Simultaneous Kidney/Bone Marrow Transplantation1

cDNA cloning of human myeloperoxidase: decrease in myeloperoxidase mRNA upon induction of HL-60 cells.

Perioperative donor bone marrow infusion augments chimerism in heart and lung transplant recipients

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