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15 results on '"Nimgaonkar, M."'

1. Development of Gene Therapy for Gaucher Disease

Author

Barranger, J.A., primary, Rice, E.O., additional, Dunigan, J., additional, Eljanne, M., additional, Takiyama, N., additional, Nimgaonkar, M., additional, Mierski, J., additional, Beeler, M., additional, Kemp, A., additional, Lancia, J., additional, Lucot, S., additional, Schierer-Fochler, S., additional, Mannion-Henderson, J., additional, Mohney, T., additional, Swaney, W., additional, Bahnson, A., additional, Bansal, V., additional, and Ball, E., additional

Published
2002
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4. A combination of CD34 selection and anti-CD15 monoclonal antibody PM-81 purging eliminates tumor cells while sparing normal progenitor cells

Author

Nimgaonkar, M., Kim, A., Lancia, J., Roscoe, R., and Ball, E.D.

Subjects
Physiological aspects, Research, Bone marrow transplantation -- Research -- Physiological aspects, Transplantation -- Research -- Physiological aspects, Cancer cells -- Physiological aspects -- Research, Organ transplantation -- Research -- Physiological aspects, Tissue transplantation -- Research -- Physiological aspects, Transplantation of organs, tissues, etc. -- Research -- Physiological aspects, Bone marrow -- Transplantation
Abstract

According to an abstract submitted by the authors to the 36th Annual Meeting of the American Society of Hematology, held December 2-6, 1994, in Nashville, Tennessee, 'Bone marrow (BM) CD34+ [...]

Published
1995

5. Immunophenotyping suggests that umbilical cord blood (CB) cells contain a high proportion of multipotential CD34+ stem cells

Author

Winkelstein, A., Nimgaonkar, M., Roscoe, R.A., Rybka, W., Hamilton, P., Dracker, R., and Ball, E.D.

Subjects
Analysis, Measurement, Bone marrow transplantation -- Analysis -- Measurement, Fetal blood -- Analysis -- Measurement, Stem cells -- Measurement -- Analysis, Bone marrow -- Transplantation
Abstract

According to an abstract submitted by the authors to the 47th annual meeting of the American Association of Blood Banks, held November 12-17, 1994, in San Diego, California, 'Background: Immunophenotyping [...]

Published
1995

6. Methods for Retrovirus-Mediated Gene Transfer to CD34(+) Enriched Cells.

Author

Bahnson AB, Nimgaonkar M, Ball ED, and Barranger JA

Abstract

Hematopoietic stem cells (HSC) provide for contmuous replenishment of the entire immune and hematopoietic systems, and also replenish themselves in a process termed self-renewal (1).The HSCs can be enriched from hematopoietic tissues using MAbs that bind to the CD34 antigen, a universally recognized marker for hematopoietic progenitors (2-4).Enriched HSC populations are being widely investigated for use in transplantation and gene therapy because they appear to provide rapid hematopoietic reconstitution in myeloablated patients (5-11), and they offer good targets for gene transfer (12-17).

Published
1997
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7. Human dendritic cells genetically engineered to express high levels of the human epithelial tumor antigen mucin (MUC-1).

Author

Henderson RA, Nimgaonkar MT, Watkins SC, Robbins PD, Ball ED, and Finn OJ

Subjects
Antigens, CD34 analysis, Hematopoietic Stem Cells cytology, Humans, Immunotherapy, Lymphocyte Activation, T-Lymphocytes immunology, Antigens, Neoplasm biosynthesis, Dendritic Cells metabolism, Genetic Engineering, Mucin-1 biosynthesis
Abstract

We have achieved stable high-level expression of a human tumor antigen, epithelial cell mucin (MUC-1), on human dendritic cells (DCs) by retroviral transduction of CD34+ progenitor cells and their subsequent cytokine-induced differentiation into DCs. The process of retroviral transduction did not alter the growth or differentiation of DCs from CD34+ progenitor cells. Immunofluorescence and electron microscopy studies revealed that the expression of mucin was limited to the body of the DCs and was excluded from the cytoplasmic veils of the DCs. Furthermore, the expression of mucin on DCs was similar, if not identical, to the nonpolarized expression of mucin found on carcinoma cells. In functional studies, the MUC-1(+)-transduced DCs were potent stimulators of allogeneic CD4+ T cells and, in fact, were superior to MUC-1- DCs. Thus, MUC-1+ DCs are expected to be a valuable tool in the immunotherapeutic treatment of patients with tumors that express MUC-1.

Published
1996

8. A combination of CD34 selection and complement-mediated immunopurging (anti-CD15 monoclonal antibody) eliminates tumor cells while sparing normal progenitor cells.

Author

Nimgaonkar M, Kemp A, Lancia J, and Ball ED

Subjects
Bone Marrow Transplantation, Cell Separation methods, Flow Cytometry, Hematopoietic Stem Cells immunology, Humans, Leukemia, Myeloid therapy, Reference Values, Tumor Cells, Cultured, Tumor Stem Cell Assay, Antibodies, Monoclonal therapeutic use, Antigens, CD34 analysis, Antigens, Neoplasm immunology, Bone Marrow Purging methods, Complement System Proteins physiology, Lewis X Antigen immunology
Abstract

Autologous bone marrow transplantation (ABMT) for acute myeloid leukemia (AML) in first complete remission (CR) results in a prolonged disease-free survival (DFS) of 34%-57%. Relapse of the underlying disease is the major cause for failure of ABMT. Relapse can result fom tumor cells either surviving in the patient or reinfused in the autograft. Genetic marking of autografted cells has demonstrated that transplanted cells contribute to relapse. This finding supports the use of purged autografts. Several purging techniques have been used. Immunologic purging using the monoclonal antibody (mAb) PM-81 (anti-CD15) has been used by our center with a long-term DFS in 50% of AML patients. PM-81 reacts with 90% of AML patients, and we have used it for over 10 years. We have investigated a two-stage purging technique involving initial selection for CD34+ cells followed by mAb purging in bone marrow (BM) and peripheral blood stem cell (PBSC) harvests. This method achieved up to a 7 log diminution in leukemic cells and 1-4 log reduction in CD15+ cells, without a significant loss of hematopoietic progenitor cells. This double-purging technique has the advantages of cytoreduction, elimination of CD34- leukemic cells, and possible improvement in the clinical efficacy of purging by concentrating for CD34+ cells. Cytoreduction by CD34 enrichment followed by purging may facilitate the use of PBSC transplants in AML.

Published
1996
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9. Efficient retroviral mediated transfer of the glucocerebrosidase gene in CD34+ enriched umbilical cord blood human hematopoietic progenitors.

Author

Mannion-Henderson J, Kemp A, Mohney T, Nimgaonkar M, Lancia J, Beeler MT, Mierski J, Bahnson AB, Ball ED, and Barranger JA

Subjects
Base Sequence, Cells, Cultured, DNA analysis, Gene Expression, Granulocytes enzymology, Humans, Macrophages enzymology, Molecular Sequence Data, Polymerase Chain Reaction, Antigens, CD34 analysis, Fetal Blood cytology, Gene Transfer Techniques, Glucosylceramidase genetics, Hematopoietic Stem Cells enzymology, Retroviridae genetics
Abstract

Obtaining efficient transfer of a normal gene and its sustained expression in self-renewing hematopoietic stem cell populations is a central concern for gene therapy initiatives. Potentially, 10(8) to 10(9) CD34+ enriched cells per patient will be required for transduction and subsequent reimplantation. These studies present an efficient method for the transduction of human CD34+ cells that can be used in a clinical study of gene transfer. The method uses a centrifugation-enhanced technique for the retroviral-mediated transfer of the normal human glucocerebrosidase (GC) gene to human CD34+ enriched umbilical cord blood cells (CB). Previous studies had described high expression of GC in CD34+ enriched cells but had not reported transduction efficiency in the progenitor population specifically. The data demonstrate an average transduction efficiency in the progenitor cell population of 50% as measured by polymerase chain reaction (PCR) for the integrated GC-cDNA in clonogenic cells. Measurements of enzyme activity comparing transduced and nontransduced fractions at 6 days posttransduction indicate an average enzyme increase of six-fold over normal background levels. PCR of colony forming units-granulocyte/macrophage (CFU-GM) plated at 6 weeks from long-term culture-initiating cell (LTC-IC) cultures also indicates transfer of the transgene to early progenitor cells. Finally, experiments were carried out with the human erythroleukemia cell line, TF-1, to estimate the durable expression of the transgene. Enzymatic activities in transduced TF-1 cultures remained at 30-fold above the activity of nontransduced controls. The expression persisted for 6 weeks in culture. These studies demonstrate efficient transduction of early progenitor cells and sustained expression of the transgene in cell cultures.

Published
1995

10. Cytokine mobilization of peripheral blood stem cells in patients with Gaucher disease with a view to gene therapy.

Author

Nimgaonkar M, Mierski J, Beeler M, Kemp A, Lancia J, Mannion-Henderson J, Mohney T, Bahnson A, Rice E, and Ball ED

Subjects
Adult, Antigens, CD34 analysis, Cell Count, Female, Gaucher Disease enzymology, Gene Transfer Techniques, Granulocyte Colony-Stimulating Factor therapeutic use, Hematopoietic Stem Cell Transplantation, Humans, Leukapheresis, Male, Middle Aged, Retroviridae genetics, Cytokines therapeutic use, Gaucher Disease blood, Gaucher Disease therapy, Genetic Therapy, Glucosylceramidase genetics, Hematopoietic Stem Cells cytology
Abstract

As clinical trials for gene therapy in Gaucher disease (GD) begin, questions regarding the biology of the hematopoietic stem cell in this disease remain unanswered. This study demonstrates the ability to mobilize and collect CD34+ cells in three patients with the disorder. Our RAC/FDA-approved clinical trial utilizes mobilized peripheral blood stem cells (PBSC) as the target cells for gene transfer. In this approach, a white blood cell fraction is collected by apheresis, enriched for CD34+ cells, and transduced with a retroviral vector carrying the glucocerebrosidase (GC) gene. Transduced cells from the patient with activity corrected to at least normal levels will be returned to the patient without myelosuppressive therapy. We report here the effect of cytokines in mobilizing PBSC in three patients with GD. Two (patients 1 and 2) were given granulocyte colony-stimulating factor (G-CSF) at a dose of 5 micrograms/kg/d and one (patient 3) was given 10 micrograms/kg/d for 10 days. Leukaphereses were done daily for 5 days and the products enriched for CD34+ cells using the clinical Ceprate (CellPro) column. The CD34+ cells in all fractions were monitored daily during mobilization and leukaphereses. Subset analysis for the expression of Thy-1, CD38, HLA-DR, and CD33 on the CD34+ cells was performed. An increase in CD34+ cells in the peripheral blood was noted from day 5 onward (up to a six-fold increase). Up to a 625-fold enrichment in CD34+ cells in the apheresis product was noted using the clinical Ceprate column. Totals of 1.2, 3.5, and 2.1 x 10(6) CD34+ cells/kg were collected in the three patients. A diminution in the percent of CD34+/Thy-1+ cells was noted with enrichment. In vitro retroviral transduction of the CD34-enriched cells using centrifugation promoted transduction protocol previously described (Bahnson AB et al., Centrifugal enhancement of retroviral-mediated gene transfer. Journal of Virology Methods 54:131, 1995) and modified for clinical use, demonstrated a mean transduction efficiency of 37% (range 8.3-87.1%) in clonogenic cells and up to 50% in long-term culture-initiating cells (LTC-IC) at week 6. Significantly, we have been able to achieve up to a 50-fold increase in the level of GC above deficient levels in the patients' CD34+ enriched cells when maintained in vitro in culture. The study demonstrates that up to a six-fold increase in CD34+ cells in the PB can be achieved with cytokines in patients with GD. CD34+ cells can be collected in numbers sufficient for conventional transplantation and transduced efficiently in vitro. In gene therapy trials for genetic disorders to date, myelosuppressive therapy is not advocated. The clinical trial will demonstrate whether this number of transduced CD34+ cells will be adequate for competitive engraftment of genetically corrected PBSC.

Published
1995

11. Long-term expression of the glucocerebrosidase gene in mouse and human hematopoietic progenitors.

Author

Nimgaonkar M, Bahnson A, Kemp A, Lancia J, Mannion-Henderson J, Boggs S, Mohney T, Baysal B, Dunigan J, and Barranger JA

Subjects
Animals, Base Sequence, Bone Marrow Cells, Colony-Forming Units Assay, DNA Primers, Fetal Blood, Gaucher Disease therapy, Hematopoietic Stem Cells enzymology, Humans, Infant, Newborn, Mice, Molecular Sequence Data, Polymerase Chain Reaction, Recombinant Proteins biosynthesis, Transduction, Genetic, Gene Expression, Genetic Therapy methods, Glucosylceramidase biosynthesis, Glucosylceramidase genetics, Hematopoietic Stem Cells cytology, Transfection
Abstract

Gaucher disease (GD), one of the most common inherited metabolic disorders, is an excellent candidate for gene therapy using hematopoietic stem cells as targets. Animal models have demonstrated the feasibility of introducing the human glucocerebrosidase (GC) gene into hematopoietic progenitors with long term expression using a variety of retroviral vectors. We have previously demonstrated the expression and integration of the human GC gene in mouse hematopoietic progenitors and their progeny 4-8 months post transplant in primary recipients using the retroviral vector MFG-GC. We now demonstrate enzyme expression in peripheral blood lymphocytes of secondary recipients more than 12 months post transplantation. We also show a transduction efficiency of up to 95% in colony forming unit-granulocyte macrophage (CFU-GM) colonies generated from transduced CD34+ cells from a variety of sources, using a centrifugation promoted infection protocol. Transduction has also been documented in long term culture initiating cells (LTCIC) from the same transduced CD34+ cells. These data indicate efficient transduction of mouse hematopoietic progenitors as well as human CD34+ cells using the retroviral vector MFG-GC.

Published
1995

12. Centrifugal enhancement of retroviral mediated gene transfer.

Author

Bahnson AB, Dunigan JT, Baysal BE, Mohney T, Atchison RW, Nimgaonkar MT, Ball ED, and Barranger JA

Subjects
3T3 Cells, Animals, Antigens, CD34, Cell Line, Fibroblasts cytology, Humans, Leukemia, Erythroblastic, Acute, Mice, Tumor Cells, Cultured, Centrifugation, Gene Transfer Techniques, Retroviridae genetics
Abstract

Centrifugation has been used for many years to enhance infection of cultured cells with a variety of different types of viruses, but it has only recently been demonstrated to be effective for retroviruses (Ho et al. (1993) J. Leukocyte Biol. 53, 208-212; Kotani et al. (1994) Hum. Gene Ther. 5, 19-28). Centrifugation was investigated as a means of increasing the transduction of a retroviral vector for gene transfer into cells with the potential for transplantation and engraftment in human patients suffering from genetic disease, i.e., gene therapy. It was found that centrifugation significantly increased the rate of transduction into adherent murine fibroblasts and into non-adherent human hematopoietic cells, including primary CD34+ enriched cells. The latter samples include cells capable of reconstitution of hematopoiesis in myeloablated patients. As a step toward optimization of this method, it was shown that effective transduction is: (1) achieved at room temperature; (2) directly related to time of centrifugation and to relative centrifugal force up to 10,000 g; (3) independent of volume of supernatant for volumes > or = 0.5 ml using non-adherent cell targets in test tubes, but dependent upon volume for coverage of adherent cell targets in flat bottom plates; and (4) inversely related to cell numbers per tube using non-adherent cells. The results support the proposal that centrifugation increases the reversible binding of virus to the cells, and together with results reported by Hodgkin et al. (Hodgkin et al. (1988) J. Virol. Methods 22, 215-230), these data support a model in which the centrifugal field counteracts forces of diffusion which lead to dissociation during the reversible phase of binding.

Published
1995
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13. A unique population of CD34+ cells in cord blood.

Author

Nimgaonkar MT, Roscoe RA, Persichetti J, Rybka WB, Winkelstein A, and Ball ED

Subjects
Antigens, CD analysis, Antigens, CD34, Bone Marrow Cells, Female, Fetal Blood immunology, Flow Cytometry, Hematopoietic Stem Cells immunology, Humans, Mucins blood, Placenta, Pregnancy, Antigens, CD blood, Fetal Blood cytology, Hematopoietic Stem Cells cytology
Abstract

Human umbilical cord blood (CB) is a rich source of hematopoietic stem cells for both research and stem cell transplantation. In clinical studies, it appears that recovery from myeloablative therapy using CB requires significantly fewer cells than a typical allogeneic marrow transplant. This suggests that CB may be enriched for early hematopoietic progenitors. The present studies were undertaken to determine the presence of CD34+ cells in CB with the phenotypic characteristics of multipotential stem cells. In 22 CB harvests, the average percentage of CD34+ cells was 1.33 +/- 0.21% (SE), a value similar to that in adult normal bone marrows (BM). However, the distribution of CD34+ cells was distinctly different from either BM or granulocyte colony-stimulating factor (G-CSF) mobilized peripheral blood stem cell harvests. CB contained a defined population of brightly staining CD34+ cells with low side scatter. These CD34 (bright) cells comprised a mean of 14.5 +/- 2.5% of the CB CD34+ cells, whereas < 1% of BM CD34+ cells has been shown to be CD34- bright. Eighty-five to ninety percent were negative for three antigens expressed at an early stage of stem cell maturation: CD38, HLA-DR and LFA-1. Fifty-five percent of these CD34 (bright) cells did not express the CD45RA isoform, an additional marker of immaturity. The antigen-bright cells also lacked lineage-specific antigens including CD33, CD56, CD19, CD10 and CD7 as well as CD71. Approximately 46% were Thy-1+, and 40% expressed c-kit receptors. These data suggest that, by phenotypic criteria, CB may be a particularly enriched source of primitive hematopoietic precursors.

Published
1995
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14. Transduction of CD34+ enriched cord blood and Gaucher bone marrow cells by a retroviral vector carrying the glucocerebrosidase gene.

Author

Bahnson AB, Nimgaonkar M, Fei Y, Boggs SS, Robbins PD, Ohashi T, Dunigan J, Li J, Ball ED, and Barranger JA

Subjects
Antigens, CD34 metabolism, Bone Marrow enzymology, Bone Marrow pathology, Fetal Blood cytology, Fetal Blood immunology, Gaucher Disease enzymology, Gaucher Disease pathology, Genetic Therapy, Humans, In Vitro Techniques, Infant, Newborn, Fetal Blood enzymology, Gaucher Disease therapy, Genetic Vectors, Glucosylceramidase genetics, Retroviridae genetics, Transduction, Genetic
Abstract

One promising strategy for gene therapy of Gaucher disease involves ex vivo retroviral transduction of autologous hematopoietic stem cells. Studies in small animals have demonstrated that this approach provides a life-long supply of the glucocerebrosidase (GC) enzyme. Human application has developed to the stage of a clinical trial. In this study, we describe development of a high titer amphotropic producer line for the vector, MFG-GC, and explore transduction of CD34+ cells from various human sources. Higher than three times the normal levels of glucocerebrosidase activity in non-transduced cells were achieved following transduction of CD34+ cells obtained from bone marrow or cord blood from normal donors. The improvement in enzyme activity in Gaucher marrow was about 40-fold above deficient levels. We examined the timing and stepwise effect of multiple rounds of infection and evaluated post-infection expansion of cells in two different cytokine mixtures. Transduction efficiency was determined using immunocytochemistry and Southern blot hybridization.

Published
1994

15. Transduction of mobilized peripheral blood CD34+ cells with the glucocerebrosidase cDNA.

Author

Nimgaonkar MT, Bahnson AB, Boggs SS, Ball ED, and Barranger JA

Subjects
Antigens, CD34 metabolism, Blood Cells enzymology, Blood Cells immunology, Gaucher Disease enzymology, Gaucher Disease genetics, Gene Expression, Gene Transfer Techniques, Genetic Therapy, Genetic Vectors, Hematopoietic Stem Cells enzymology, Hematopoietic Stem Cells immunology, Humans, In Vitro Techniques, Retroviridae genetics, DNA, Complementary genetics, Gaucher Disease therapy, Glucosylceramidase genetics, Transduction, Genetic
Abstract

Gaucher disease (GD), the most common human lysosomal storage disorder, results from a genetic deficiency of the enzyme glucocerebrosidase (GC). The cloning of human GC cDNA, the benefits of allogeneic bone marrow transplantation and the success of enzyme replacement therapy support the feasibility of gene therapy as an approach to a cure for GD. We report the transfer of the GC gene to mobilized human peripheral blood (PB) CD34+ cells obtained from patients primed with granulocyte colony-stimulating factor and/or chemotherapy. A tenfold enrichment of CD34+ cells was achieved using an avidin-biotin immunoadsorption technique. Prestimulation of the CD34+ cells with cytokines, followed by infection for 5 days with a supernatant containing the MFG-GC retroviral vector, resulted in enzyme activity up to 2.5-times greater than non-infected and lac-Z infected controls. Southern blot hybridization of DNA from these cells demonstrated a transduction efficiency of 10-30%. These studies show that the GC gene is transferred efficiently to mobilized PB CD34+ cells by the MFG-GC retroviral vector and results in expression of enzyme activity in the population of cells capable of bone marrow reconstitution. These results advance the development of gene therapy for GD.

Published
1994

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