Your search keyword '"Yang, Z. Y."' showing total 12 results

1. Genetic vaccination-induced immune responses to the human immunodeficiency virus protein Rev: emergence of the interleukin 2-producing helper T lymphocyte.

Author

Chan SY, Louie MC, Piccotti JR, Iyer G, Ling X, Yang ZY, Nabel GJ, and Bishop DK

Subjects

Animals, Cytokines biosynthesis, Enzyme-Linked Immunosorbent Assay, Female, Immunoglobulin G biosynthesis, Lymphocyte Activation, Mice, Mice, Inbred BALB C, Mice, Inbred C57BL, Plasmids genetics, Spleen immunology, T-Lymphocyte Subsets immunology, Transforming Growth Factor beta genetics, Transgenes, Vaccination, Gene Products, rev genetics, Gene Products, rev immunology, Gene Transfer Techniques, Interleukin-2 biosynthesis, T-Lymphocytes, Helper-Inducer immunology

Abstract

Rev M10 is a trans-dominant negative inhibitor of HIV replication. Hence, stable transduction of CD4+ T cells with Rev M10 represents a novel gene therapy aimed at inhibiting HIV replication within these cells, thereby slowing the progression of AIDS. However, the immune system may recognize Rev M10 as foreign and target transduced cells for elimination. In the current study, mice were genetically immunized with a plasmid encoding Rev M10, to (1) identify immune parameters that may be induced by Rev M10 gene transfer, (2) determine the impact of repeated introduction of the Rev M10-encoding plasmid on the immune response to the transgene product, and (3) determine if cotransfection with a plasmid encoding TGFbeta1 would suppress the response. Kinetic studies revealed that Rev-specific IL-2-producing helper T lymphocytes (HTLs) appeared following the second genetic immunization, peaked after the third, and persisted at peak levels for at least 6 weeks. Rev-specific HTLs were CD4+, and the development of these cells was ablated by cotransfection with TGFbeta1. Other cytokines were not readily detectable when immune splenocytes were restimulated with Rev in vitro, and Rev-specific IgG antibodies were not present in the sera of these mice. To our knowledge, this represents the first report that genetic immunization with Rev M10 induces an immune response that is dominated by IL-2-producing HTLs. Further, this study demonstrates the potential utility of introducing immunosuppressive genes as a means to control the immune response to foreign transgene products.

Published

1998

2. Gene transfer into human umbilical cord blood-derived CD34+ cells by particle-mediated gene transfer.

Author

Verma S, Woffendin C, Bahner I, Ranga U, Xu L, Yang ZY, King SR, Kohn DB, and Nabel GJ

Subjects

Anti-Bacterial Agents, Antigens, CD34 isolation & purification, Blotting, Southern, Cell Differentiation, Cell Separation, Cells, Cultured, Chloramphenicol O-Acetyltransferase genetics, Coculture Techniques, Cytomegalovirus genetics, Drug Resistance genetics, Fetal Blood cytology, Flow Cytometry, Genes, Reporter, Genetic Therapy methods, Genetic Vectors, Gentamicins pharmacology, Gold Colloid, Humans, Neomycin, Plasmids, Polymerase Chain Reaction, Antigens, CD34 genetics, Gene Transfer Techniques, Hematopoietic Stem Cells cytology, Transfection methods

Abstract

Delivery of genes into hematopoietic progenitor cells offers an attractive means for the introduction of corrective or protective genes into cells of both the myeloid and lymphoid lineage. Previously, investigators have often used murine retroviral vectors for gene delivery which require cells to be cycling for efficient delivery. We describe a nonviral method of gene delivery using particle-mediated gene transfer to obviate many disadvantages of viral vectors related to safety, production costs and the need for cell cycle proliferation. Using a CMV-CAT reporter plasmid, we show transfection of highly purified CD34+ cells isolated from umbilical cord blood. Effective gene transfer was shown in unstimulated and in growth-stimulated cells. Following transfection with a neomycin resistance gene, differentiation into cells of the myeloid lineage was observed, assayed by CFU-GM in the presence of G-418. Both unstimulated and stimulated cells gave rise to CFU-GM in the presence of G-418, indicating that stable expression of the neomycin resistance gene was maintained in early progenitors. These results demonstrate that particle-mediated gene transfer into human hematopoietic cells from umbilical cord blood can be achieved without affecting their CFU-GM differentiation potential. This gene transfer method offers an alternative approach to gene therapy studies involving human hematopoietic progenitor cells.

Published

1998

3. Inhibition of vascular smooth muscle cell proliferation and intimal hyperplasia by gene transfer of beta-interferon.

Author

Stephan D, San H, Yang ZY, Gordon D, Goelz S, Nabel GJ, and Nabel EG

Subjects

Adenoviridae genetics, Adenoviridae metabolism, Animals, Arteries injuries, Blotting, Western, Catheterization adverse effects, Cell Division, Cells, Cultured, Culture Media, Conditioned, Gene Expression Regulation, Genetic Vectors genetics, Interferon-beta therapeutic use, RNA, Messenger metabolism, Recombinant Proteins therapeutic use, Swine, Transfection genetics, Vascular Diseases therapy, Gene Transfer Techniques, Interferon-beta genetics, Muscle, Smooth, Vascular cytology

Abstract

Background: Balloon injury of the arterial wall induces increased vascular smooth cell proliferation, enhanced elastic recoil, and abnormalities in thrombosis, each of which contribute to regrowth of intima and the lesion of restenosis. Several gene transfer approaches have been used to inhibit such intimal smooth muscle cell growth. In this report, adenoviral gene transfer of beta-interferon (beta-IFN) was analyzed in a porcine model of balloon injury to determine whether a secreted growth inhibitory protein might affect the regrowth of vascular smooth muscle cells in vitro and in arteries., Materials and Methods: An adenoviral vector encoding beta-interferon (ADV-beta-IFN) was prepared and used to infect porcine vascular smooth muscle cells in a porcine balloon injury model. Its antiproliferative effect was analyzed in vitro and in vivo., Results: Expression of recombinant porcine beta-IFN in vascular smooth muscle cells reduced cell proliferation significantly in vitro, and supernatants derived from the beta-IFN vector inhibited vascular smooth muscle cell proliferation relative to controls. When introduced into porcine arteries after balloon injury, a reduction in cell proliferation was observed 7 days after gene transfer measured by BrdC incorporation (ADV-delta E1 arteries 14.5 +/- 1.2%, ADV-beta IFN 6.8 +/- 0.8%, p < 0.05, unpaired, two-tailed t-test). The intima-to-media area ratio was also reduced (nontransfected arteries, 0.70 +/- 0.05; ADV-delta E1 infected arteries, 0.69 +/- 0.06; ADV-beta-IFN infected arteries, 0.53 +/- 0.03; p < 0.05, ANOVA with Dunnett t-test). No evidence of organ toxicity was observed, and regrowth of the endothelial cell surface was observed 3-6 weeks after balloon injury., Conclusions: Gene transfer of an adenoviral vector encoding beta-IFN into balloon-injured arteries reduced vascular smooth muscle proliferation and intimal formation. Expression of this gene product may have potential application for the treatment of vascular proliferative diseases.

Published

1997

4. A new cationic liposome DNA complex enhances the efficiency of arterial gene transfer in vivo.

Author

Stephan DJ, Yang ZY, San H, Simari RD, Wheeler CJ, Felgner PL, Gordon D, Nabel GJ, and Nabel EG

Subjects

Animals, Drug Carriers metabolism, Ethers metabolism, Female, Gene Expression Regulation, Male, Mice, Phosphatidylethanolamines metabolism, Quaternary Ammonium Compounds metabolism, Swine, Transfection methods, DNA metabolism, Gene Transfer Techniques, Liposomes metabolism

Abstract

An important goal of gene therapy for cardiovascular diseases and cancer is the development of effective vectors for catheter-based gene delivery. Although adenoviral vectors have proven effective for this purpose in animal models, the ability to achieve comparable gene transfer with nonviral vectors would provide potentially desirable safety and toxicity features for clinical studies. In this report, we describe the use of a new cationic DNA-liposome complex using an improved expression vector and lipid, N-(3-aminopropyl)-N, N-dimethyl-2,3-bis(dodecyloxy)-1-propaniminium bromide/dioleyl phosphatidylethanolamine (GAP-DL-RIE/DOPE) to optimize catheter-mediated gene transfer in porcine arteries. The efficiency of this vector was compared to DNA alone, DNA with a previously described cationic liposome complex, (+/-)-N-(2-hydroxyethyl)-N, N-dimethyl-2,3-bis(tetradecyloxy)-1-propanaminium bromide (DMRIE/DOPE), and a replication-defective adenoviral vector in a porcine artery gene transfer model. When used in optimal ratios, GAP-DL-RIE/DOPE liposomes provided a 15-fold higher level of gene expression in arteries compared to DNA alone or DMRIE/DOPE. Gene expression was observed in intimal and medial cells. However, when compared to adenoviral vectors (10(10) pfu/ml), gene expression following GAP-DLRIE/DOPE transfection was approximately 20-fold lower. Following intravenous injection of GAP-DLRIE/DOPE in mice, biochemical, hematological, and histopathological abnormalities were not observed. Significant improvements in the efficacy of arterial gene expression can be achieved by optimization of transfection condition with DNA-liposome complexes in vivo that may prove useful for arterial gene delivery in cardiovascular diseases and cancer.

Published

1996

5. [Study on the transferring of YACs to new host by means of KAR cross].

Author

Yang ZY and Kuang DR

Subjects

Crossing Over, Genetic, Genomic Library, Humans, Chromosomes, Artificial, Yeast genetics, Gene Transfer Techniques

Abstract

The donor yeast strain YAC23 containing a 340 kb human genomic DNA fragment in YAC (Yeast Artificial Chromosome) was mated with recipient strain YLB504 by means of improved kar cross and the condidate YACductants were assayed by PCR and the amplification band of 404 bp indicated that they were the same as those of recipient strains (i.e. MAT alpha). Further analysis of the electrokaryotype of the candidate YACductants by PFGE (Pulsed Field Gel Electrophoresis) confirmed that the YACs had succeeded in entering into the recipient cells. The YACs had thus completed the process of transferring from one host to the other.

Published

1996

6. Direct gene transfer for treatment of human cancer.

Author

Nabel GJ, Yang ZY, Nabel EG, Bishop K, Marquet M, Felgner PL, Gordon D, and Chang AE

Subjects

Animals, Clinical Trials, Phase I as Topic, Drug Carriers, Gene Expression Regulation, Neoplastic, HLA-B7 Antigen immunology, Humans, Injections, Intralesional, Liposomes, Male, Mice, Neoplasms immunology, DNA, Recombinant administration & dosage, Gene Transfer Techniques, Genes, MHC Class I, HLA-B7 Antigen genetics, Neoplasms therapy, Recombinant Fusion Proteins immunology

Abstract

Genetic instability within malignant cells gives rise to mutant proteins which can be recognized by the immune system. Recognition of tumor-associated antigens by T lymphocytes could thus contribute to the elimination of neoplastic cells. We have developed a molecular genetic intervention for the treatment of malignancies based upon the knowledge that foreign major histocompatibility complex (MHC) proteins expressed on the cell surface are efficient at stimulating an immune response. Expression of this foreign MHC gene within tumors induced a cytotoxic T cell response to the introduced gene. More importantly, the immune system recognized tumor-specific antigens on unmodified tumor cells as foreign. Growth of the tumors diminished, and in many cases, there was complete regression. This research provides evidence that direct gene transfer in vivo can induce cell-mediated immunity against specific gene products, and offers the potential for effective immunotherapy for the treatment of cancer and infectious diseases in man. Our laboratory conducted a phase I clinical trial to determine the safety and efficacy of this treatment in humans. These studies suggest that direct gene transfer provides a safe and feasible approach for the treatment of human cancer. More recent developments using combination gene therapy and the initiation of a second human trial with improvements on this technology have been implemented. Finally, we have begun to define mechanisms of resistance to immune recognition by established malignancies.

Published

1995

7. Genetic modification of human peripheral blood lymphocytes with a transdominant negative form of Rev: safety and toxicity.

Author

Fox BA, Woffendin C, Yang ZY, San H, Ranga U, Gordon D, Osterholzer J, and Nabel GJ

Subjects

Animals, Antiviral Agents pharmacology, Base Sequence, Cell Line, Cell Transformation, Neoplastic, Cytokines biosynthesis, Female, Fibroblasts, Genes, Dominant, Gold toxicity, HIV-1 physiology, Humans, Immunotherapy, Adoptive, Interleukin-2 physiology, Lymphocyte Activation, Mice, Mice, Inbred BALB C, Mice, SCID, Microspheres, Molecular Sequence Data, Retroviridae genetics, Reverse Transcriptase Inhibitors pharmacology, T-Lymphocytes metabolism, T-Lymphocytes transplantation, Virus Replication drug effects, Gene Transfer Techniques, Genes, rev genetics, Genetic Vectors, HIV-1 genetics, T-Lymphocytes immunology

Abstract

A transdominant mutant form of the rev gene, M10, confers resistance to infection by the human immunodeficiency virus (HIV) in vitro and is currently under investigation as a potential intervention in acquired immunodeficiency syndrome (AIDS). In this report, we examine three issues relevant to the safety of autologous transfer of human T cells genetically modified with Rev M10. First, the potential for malignant transformation was assessed in vitro using interleukin-2 (IL-2) dependence and fibroblast transformation assays, and tumorigenicity was evaluated in severe combined immunodeficient (SCID) mice. Possible toxicity was evaluated by pathologic analysis following adoptive transfer of genetically modified human T cells into SCID mice. Second, methods were developed that permit T cell activation required for gene transfer but do not allow replication of endogenous HIV. Third, T cell function was evaluated in peripheral blood lymphocytes (PBL) of HIV-seropositive donors transduced with Rev M10 and compared to a negative control mutant, delta Rev M10. By all criteria, no oncogenicity or toxicity was observed. Human T cells transduced with these vectors did not grow in the absence of IL-2 in vitro, and no tumors were observed following transplantation of genetically modified human cells into recipient SCID mice. Histopathological analysis of heart, lung, liver, spleen, and kidney of animals 1-21 weeks following adoptive transfer of gene-modified human T cells revealed no significant abnormalities. Additionally, no differences were observed in the pattern of cytokine secretion in enriched human PBL expressing Rev M10 compared to delta Rev M10. (ABSTRACT TRUNCATED AT 250 WORDS)

Published

1995

8. Nonviral and viral delivery of a human immunodeficiency virus protective gene into primary human T cells.

Author

Woffendin C, Yang ZY, Udaykumar, Xu L, Yang NS, Sheehy MJ, and Nabel GJ

Subjects

Base Sequence, Cells, Cultured, DNA Primers chemistry, Genes, Dominant, Genes, Suppressor, Gold, Humans, In Vitro Techniques, Molecular Sequence Data, Transduction, Genetic, Transfection, Virus Replication, rev Gene Products, Human Immunodeficiency Virus, Gene Products, rev administration & dosage, Gene Transfer Techniques, Genes, rev, Genetic Therapy, HIV Infections prevention & control, HIV-1 genetics, T-Lymphocytes microbiology

Abstract

Because AIDS has been refractory to traditional pharmacologic interventions, alternative approaches have been developed. Although the introduction of specific antiviral genes into T leukemia cells can provide relative resistance to human immunodeficiency virus (HIV) replication, the testing of such genes against primary viral isolates in human CD4+ lymphocytes has been limited, and safety questions remain regarding gene delivery into cells from HIV-infected patients. In this report, we evaluate the efficacy of a transdominant mutant protein, Rev M10, against cloned and primary HIV isolates in human peripheral blood lymphocytes and describe different methods of gene transfer into peripheral blood lymphocytes from HIV-infected individuals. We show that gold microparticles can mediate stable Rev M10 gene transfer into these cells. Introduction of Rev M10 by these techniques conferred resistance to HIV infection in vitro to cloned and clinical isolates. Nonviral delivery of HIV protective genes will facilitate the development of gene therapy for AIDS and the analysis of viral and cellular gene expression in human T lymphocytes.

Published

1994

9. Direct gene transfer for the understanding and treatment of human disease.

Author

Plautz GE, Nabel EG, Fox B, Yang ZY, Jaffe M, Gordon D, Chang A, and Nabel GJ

Subjects

Animals, Autoimmunity, Blood Vessels, Cations, Genetic Vectors, H-2 Antigens genetics, Histocompatibility Antigens Class I genetics, Humans, Liposomes, Mice, Neoplasms immunology, Retroviridae genetics, Swine, Gene Transfer Techniques, Genetic Therapy

Abstract

Direct gene transfer has been used to develop molecular genetic interventions for acquired diseases in several animal models. Through the use of intravascular catheters or anatomically localized injection of DNA liposome complexes, specific tissues can be transduced with recombinant genes. Several promising applications of this method for the study of vascular biology have been demonstrated by direct gene transfer into arteries in vivo. Delivery, via catheter, of genes that modulate the thrombogenic or proliferative properties of vascular cells may someday provide therapy for stenotic lesions of atherosclerosis or following angioplasty. Cancer is another acquired disorder in which direct gene transfer may improve the efficacy of treatment. Introduction of class I MHC or cytokine genes with antitumor or immunostimulatory effects have demonstrated promise in animal models. Direct transfer of an allogeneic class I MHC gene into tumors in vivo induces a CD8+ CTL response against weak antigens on poorly immunogenic tumors. The efficacy of this antitumor response can be augmented to induce regression of actively growing established tumors. Additional strategies, such as intratumoral delivery of combinations of multiple cytokine and MHC genes, may serve to improve the antitumor response. A clinical gene therapy protocol is underway to analyze the safety and efficacy of DNA liposome-mediated gene transfer in humans. Development of improved gene delivery systems and introduction of recombinant genes into visceral tumors by intravascular catheter will extend the application of direct gene transfer to immunotherapy of malignancies. These clinical trials of direct gene transfer will help to develop new treatment strategies for human diseases.

Published

1994

10. Direct gene transfer with DNA-liposome complexes in melanoma: expression, biologic activity, and lack of toxicity in humans.

Author

Nabel GJ, Nabel EG, Yang ZY, Fox BA, Plautz GE, Gao X, Huang L, Shu S, Gordon D, and Chang AE

Subjects

Aged, Base Sequence, Cytotoxicity, Immunologic, DNA Primers chemistry, Female, Gene Expression Regulation, Neoplastic, Genes, MHC Class I, Genetic Therapy, HLA-B7 Antigen genetics, Humans, Liposomes, Male, Middle Aged, RNA, Messenger genetics, DNA administration & dosage, Gene Transfer Techniques, Melanoma therapy, Skin Neoplasms therapy

Abstract

Direct gene transfer offers the potential to introduce DNA encoding therapeutic proteins to treat human disease. Previously, gene transfer in humans has been achieved by a cell-mediated ex vivo approach in which cells from the blood or tissue of patients are genetically modified in the laboratory and subsequently returned to the patient. To determine the feasibility and safety of directly transferring genes into humans, a clinical study was performed. The gene encoding a foreign major histocompatibility complex protein, HLA-B7, was introduced into HLA-B7-negative patients with advanced melanoma by injection of DNA-liposome complexes in an effort to demonstrate gene transfer, document recombinant gene expression, and determine the safety and potential toxicity of this therapy. Six courses of treatment were completed without complications in five HLA-B7-negative patients with stage IV melanoma. Plasmid DNA was detected within biopsies of treated tumor nodules 3-7 days after injection but was not found in the serum at any time by using the polymerase chain reaction. Recombinant HLA-B7 protein was demonstrated in tumor biopsy tissue in all five patients by immunochemistry, and immune responses to HLA-B7 and autologous tumors could be detected. No antibodies to DNA were detected in any patient. One patient demonstrated regression of injected nodules on two independent treatments, which was accompanied by regression at distant sites. These studies demonstrate the feasibility, safety, and therapeutic potential of direct gene transfer in humans.

Published

1993

11. Requirements for enhanced transgene expression by untranslated sequences from the human cytomegalovirus immediate-early gene

Author

Simari, R. D., Yang, Z. Y., Ling, X., Stephan, D., Perkins, N. D., Nabel, G. J., and Nabel, E. G.

Subjects

Chloramphenicol O-Acetyltransferase, Swine, Gene Transfer Techniques, Cytomegalovirus, Gene Expression, Transfection, Muscle, Smooth, Vascular, Genes, Reporter, Untranslated Regions, Animals, Humans, Promoter Regions, Genetic, Genes, Immediate-Early, Cells, Cultured, Research Article, Plasmids

Abstract

BACKGROUND: The cytomegalovirus immediate early (CMV IE) promoter has been widely used for heterologous expression. Further enhancements of gene expression from this potent promoter may allow for the development of improved gene transfer strategies. We aimed to determine whether inclusion of the first exon (5' untranslated) and first intron of the CMV IE gene would increase heterologous transgene expression in primary target cells and to determine the sequences required for any observed increases. MATERIALS AND METHODS: Comparisons of reporter gene expression were made following transient transfection of vascular smooth muscle cells (VSMCs) with plasmids containing the first exon and intron from the CMV IE gene or deletional mutations. Comparisons were also made using a heterologous promoter (RSV). RESULTS: Gene expression from the CMV IE promoter was increased 5.7-fold in VSMC with the inclusion of the first exon and intron. Similar increases were seen with other target cells and from the heterologous RSV promoter. This increase was associated with an increase in steady-state mRNA. Deletion analyses demonstrated that the enhancement was dependent on the presence of the 5' portion of the first exon while deletion of large segments within the intron was associated with similar levels of expression compared with the parental plasmid. CONCLUSIONS: Inclusion of the first exon and intron from the CMV IE gene increases expression from the CMV IE promoter. This enhancement is seen with the heterologous RSV promoter and is associated with an increase in steady-state mRNA. Deletion analyses suggest that this enhancement is associated with inclusion of sequences within the 5' portion of the first exon and inclusion of an intron.

Published

1998

12. Inhibition of vascular smooth muscle cell proliferation and intimal hyperplasia by gene transfer of beta-interferon

Author

Stephan, D., San, H., Yang, Z. Y., Gordon, D., Goelz, S., Nabel, G. J., and Nabel, E. G.

Subjects

Swine, Blotting, Western, Genetic Vectors, Gene Transfer Techniques, Arteries, Interferon-beta, Transfection, Muscle, Smooth, Vascular, Recombinant Proteins, Adenoviridae, Catheterization, Gene Expression Regulation, Culture Media, Conditioned, Animals, RNA, Messenger, Vascular Diseases, Cell Division, Cells, Cultured, Research Article

Abstract

BACKGROUND: Balloon injury of the arterial wall induces increased vascular smooth cell proliferation, enhanced elastic recoil, and abnormalities in thrombosis, each of which contribute to regrowth of intima and the lesion of restenosis. Several gene transfer approaches have been used to inhibit such intimal smooth muscle cell growth. In this report, adenoviral gene transfer of beta-interferon (beta-IFN) was analyzed in a porcine model of balloon injury to determine whether a secreted growth inhibitory protein might affect the regrowth of vascular smooth muscle cells in vitro and in arteries. MATERIALS AND METHODS: An adenoviral vector encoding beta-interferon (ADV-beta-IFN) was prepared and used to infect porcine vascular smooth muscle cells in a porcine balloon injury model. Its antiproliferative effect was analyzed in vitro and in vivo. RESULTS: Expression of recombinant porcine beta-IFN in vascular smooth muscle cells reduced cell proliferation significantly in vitro, and supernatants derived from the beta-IFN vector inhibited vascular smooth muscle cell proliferation relative to controls. When introduced into porcine arteries after balloon injury, a reduction in cell proliferation was observed 7 days after gene transfer measured by BrdC incorporation (ADV-delta E1 arteries 14.5 +/- 1.2%, ADV-beta IFN 6.8 +/- 0.8%, p < 0.05, unpaired, two-tailed t-test). The intima-to-media area ratio was also reduced (nontransfected arteries, 0.70 +/- 0.05; ADV-delta E1 infected arteries, 0.69 +/- 0.06; ADV-beta-IFN infected arteries, 0.53 +/- 0.03; p < 0.05, ANOVA with Dunnett t-test). No evidence of organ toxicity was observed, and regrowth of the endothelial cell surface was observed 3-6 weeks after balloon injury. CONCLUSIONS: Gene transfer of an adenoviral vector encoding beta-IFN into balloon-injured arteries reduced vascular smooth muscle proliferation and intimal formation. Expression of this gene product may have potential application for the treatment of vascular proliferative diseases.

Published

1997