Your search keyword '"Fabre JW"' showing total 219 results

1. Integrin-mediated transfection with peptides containing arginine-glycine-aspartic acid domains

Author

Hart, SL, Collins, L, Gustafsson, K, and Fabre, JW

Published

1997

2. Abstracts

Author

Peter J. Morris, Michael E. French, WilliamP. Homan, T. G. Denton, Peter R. Millard, Fabre Jw, and Keryn A. Williams

Subjects

business.industry, Cyclosporin a, Medicine, Surgery, Pharmacology, business, Mode of action

Published

1979

3. THE DETAILED DISTRIBUTION OF MHC CLASS II ANTIGENS IN NORMAL HUMAN ORGANS

Author

Peter J. Morris, Fabre Jw, A S Daar, A. Ting, and Susan V. Fuggle

Subjects

Male, HLA-DP Antigens, Pathology, medicine.medical_specialty, medicine.drug_class, Respiratory System, Kidney, Monoclonal antibody, Cardiovascular System, Nervous System, Antigen, HLA Antigens, Endocrine Glands, HLA-DQ Antigens, Testis, medicine, Humans, HLA-DR Antigen, Transplantation, HLA-DQ Antigen, biology, HLA-DP Antigen, Histocompatibility Antigens Class II, Antibodies, Monoclonal, HLA-DR Antigens, Staining, Lymphatic system, Immunology, biology.protein, Antibody, Digestive System

Abstract

In a previous article we described the detailed tissue distribution of MHC class I antigens. In this study, we have used a monoclonal antibody, NFK1, to study the tissue distribution of MHC class II antigens. This antibody, which detects a monomorphic determinant common to the DR, SB, and DC molecules, was used to stain frozen sections of normal tissues from throughout the human body by a sensitive peroxidase-antiperoxidase immunohistological technique. Although previous studies, both in animal models and in human beings, have shown that class II antigens are expressed on a limited number of nonlymphoid tissues, our study has extended the spectrum of tissues on which this class of antigens is detectable. Epithelial cells in a number of organs were positively stained--these include the tongue, tonsils, epiglottis, trachea, small intestine, urethra, epididymis, and proximal renal tubules. Lymphatics throughout the body appeared to express class II antigens. Capillaries in brain, testis, and placenta appeared not to express class II antigens, but in the rest of the body they showed strong and uniform staining. These and other observations, and their implications, are discussed in relation to previously published studies.

Published

1984

4. MAJOR HISTOCOMPATIBILITY COMPLEX ANTIGENS IN THE RAT PANCREAS, ISOLATED PANCREATIC ISLETS, THYROID, AND ADRENAL

Author

Mary R. Newton, Fabre Jw, Peter J. Morris, D. N. J. Hart, and H. Reece-Smith

Subjects

Male, endocrine system, medicine.medical_specialty, endocrine system diseases, medicine.drug_class, Thyroid Gland, Major histocompatibility complex, Monoclonal antibody, Major Histocompatibility Complex, Islets of Langerhans, Antigen, Histocompatibility Antigens, Internal medicine, Adrenal Glands, medicine, Animals, Pancreas, Transplantation, biology, Passenger leukocyte, Pancreatic islets, Thyroid, Antibodies, Monoclonal, Rats, Inbred Strains, Molecular biology, Rats, Histocompatibility, medicine.anatomical_structure, Endocrinology, biology.protein, Adrenal medulla

Abstract

Monoclonal antibodies to rat class I and class II MHC antigens have been used with the peroxidase-antiperoxidase technique to localize these antigens in the DA rat pancreas, isolated pancreatic islets, adrenal, and thyroid tissue. The class I (RT1A) antigens were found to be expressed by pancreatic islet cells, adrenal cortical cells, thyroid follicular cells, and--in low concentration--on cells of the adrenal medulla. These same cells did not express class II (Ia or RT1B) antigens. However, interstitial dendritic cells, staining intensely for class II antigens were present in thyroid, adrenal and pancreatic tissue, and within isolated pancreatic islets. These cells probably represent the immunogenic passenger leukocyte.

Published

1983

5. A human thymocyte antigen defined by a hybrid myeloma monoclonal antibody

Author

Cesar Milstein, David Y. Mason, Andrew J. McMichael, Fabre Jw, Giovani Galfré, and Jennifer R. Pilch

Subjects

medicine.drug_class, Immunoprecipitation, T-Lymphocytes, Immunology, Human leukocyte antigen, Hybrid Cells, Monoclonal antibody, Antibodies, Immunoenzyme Techniques, Mice, Antigen, Antibody Specificity, medicine, Animals, Chemical Precipitation, Humans, Immunology and Allergy, Antigens, Polyacrylamide gel electrophoresis, Mice, Inbred BALB C, Binding Sites, biology, Molecular biology, Clone Cells, Thymocyte, Myeloma Proteins, Macrophage-1 antigen, biology.protein, Hybridization, Genetic, Electrophoresis, Polyacrylamide Gel, Female, Antibody

Abstract

Spleen cells from a BALB/c mouse that had been immunized with human thymocytes were fused with the myeloma line P3-NS 1/1 Ag 4.1. One of the resulting hybrid clones (NA 1/34) secreted an antibody that was highly specific for human thymocytes. Eighty-five % of thymocytes expressed the antigen designated HTA1. There were an estimated 15 x 10(4) molecules of HTA 1 per cell, and it is therefore a major surface molecule. The expression of this antigen on thymocytes appears to be reciprocal to HLA, as recognized by another monoclonal antibody W6/32. Immunoprecipitated material from [125I]-labeled thymocyte membranes was analyzed by polyacrylamide gel electrophoresis in sodium dodecyl sulfate which disclosed a single component of 45,000 molecular weight.

Published

1979

6. Purification and Preliminary Biochemical Characterisation of the Human and Rat Forms of the Central Nervous System-Specific Molecule, F3-87-8

Author

Fabre Jw, A. K. Allen, and Kenneth H. Lakin

Subjects

medicine.drug_class, Carbohydrates, Biology, Monoclonal antibody, Biochemistry, Chromatography, Affinity, Epitope, Serine, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Species Specificity, medicine, Animals, Humans, Amino Acids, Threonine, Polyacrylamide gel electrophoresis, Glycoproteins, Brain Chemistry, chemistry.chemical_classification, Antibodies, Monoclonal, Carbohydrate, Molecular biology, Rats, Amino acid, Sialic acid, Molecular Weight, chemistry, Electrophoresis, Polyacrylamide Gel

Abstract

The F3-87-8 monoclonal antibody recognises a phylogenetically conserved antigenic determinant found exclusively in the mammalian CNS. We used this monoclonal antibody as the major purification step for obtaining pure. F3-87-8-bearing molecules from rat and human brains for biochemical analysis. In both rat and man, the F3-87-8 molecule is a heavily glycosylated protein, consisting of 47.6 and 47.0% carbohydrate by weight, respectively. In both species, it occurs as a doublet on polyacrylamide gel electrophoresis in sodium dodecyl sulphate, the Mr of the human form being 130,000 and 100,000. In the rat, the Mr of the doublet is slightly but consistently lower than in man, and the higher-Mr band is more pronounced. The amino acid composition of the rat and human forms is virtually identical, with a high content of serine and threonine. Significant differences are seen in carbohydrate composition, the rat form containing more sialic acid and neutral sugar and less hexosamine than the human form. beta-Elimination studies, in conjunction with carbohydrate analysis, suggest the presence of approximately 40 O-linked and 10-15 N-linked oligosaccharides per polypeptide chain of 500 amino acids, the N-linked chains predominantly of the high-mannose type. This makes it likely that the molecule adopts an extended rather than a coiled conformation on the membrane.

Published

1983

7. LOCALIZATION OF MAJOR HISTOCOMPATIBILITY COMPLEX (HLA-ABC AND DR) ANTIGENS IN 46 KIDNEYS

Author

Fabre Jw, Peter J. Morris, Susan V. Fuggle, P Errasti, A. Ting, and A S Daar

Subjects

Adult, Male, Pathology, medicine.medical_specialty, Adolescent, Endothelium, Kidney Glomerulus, Human leukocyte antigen, Kidney, Major histocompatibility complex, Antigen, HLA Antigens, HLA-DR, Humans, Medicine, Transplantation, biology, urogenital system, business.industry, Histocompatibility Antigens Class II, HLA-DR Antigens, Capillaries, Kidney Tubules, medicine.anatomical_structure, Mesangium, Immunology, biology.protein, Female, Antibody, business

Abstract

Biopsies from 46 kidneys that were subsequently transplanted were examined with monoclonal antibodies and the peroxidase-antiperoxidase technique to localize HLA-ABC and DR antigens. There was no variation in the expression of HLA-ABC which was present on all cells of the renal parenchyma. HLA-DR was found consistently on the endothelium of glomeruli and of intertubular capillaries but was only weakly expressed, or not expressed at all, on the endothelium of large vessels. The mesangium of glomeruli also stained for HLA-DR. But there was a striking variation in the expression of HLA-DR by proximal renal tubular cells in the 46 kidneys. HLA-DR was absent from tubules in 11 of 46 kidneys (23%) and probably absent or very weakly expressed in a further 8 kidneys (17%). The expression of HLA-DR in tubular epithelium was not related to the donor's age, sex, blood group, or ischemia times. However, the frequency of HLA-DR3 increased (55%) in donors of kidneys with tubular DR-negative kidneys, as compared with a frequency of 15% in donors of tubular DR-positive kidneys. Although this difference was not significant after a correction for the number of comparisons made, it suggests a genetic influence on the expression of tubular DR. The survival of tubular DR-negative kidneys was better at 1 year than that of tubular DR-positive kidneys (70% vs. 57%--not significant), and tubular DR-positive grafts may have had a higher rate of delayed function when transplanted in cases with a donor-specific positive B cell crossmatch. There was no obvious variation in the number of dendritic cells stained with antibodies to HLA-DR and the leukocyte common antigen despite prior administration of high doses of steroids to some donors before nephrectomy.

Published

1983

8. STUDIES ON THE IMMUNOSUPPRESSIVE PROPERTIES OF CYCLOSPORIN A IN RATS RECEIVING RENAL ALLOGRAFTS

Author

Peter R. Millard, Fabre Jw, William P. Homan, Peter J. Morris, and Keryn A. Williams

Subjects

Cytotoxicity, Immunologic, Male, Immunity, Cellular, Transplantation, Dose-Response Relationship, Drug, business.industry, Graft Survival, Drug Evaluation, Preclinical, Cyclosporins, Pharmacology, Kidney Transplantation, Peptides, Cyclic, Rats, Time, Histocompatibility, Lethal Dose 50, Rats, Inbred Lew, Cyclosporin a, Renal allograft, Animals, Transplantation, Homologous, Medicine, business, Immunosuppressive Agents

Abstract

The immunosuppressive effects of cyclosporin A were tested in a DA (RT-1a) to Lewis (RT-1(1) rat renal allograft model, which represents a very strong histocompatibility barrier. Dose-response studies established that oral doses of 5 mg/kg/day or higher gave complete suppression of rejection, while oral doses of 2 mg/kg/day or lower were without effect. Intravenous administration of the drug approximately doubled its potency. Time studies showed that the period of administration was also critical, with a 7- or 14-day treatment course with 5 mg/kg/day orally giving prolonged graft survival, while a 4-day course was without effect. Large doses (up to 25 mg/kg/day orally) from day 4 after transplantation did not prolong graft survival, suggesting that cyclosporin A has no effect on an established rejection response. It was found that the lymphocytotoxin response to the graft was markedly suppressed by doses of cyclosporin A which maintained normal graft function, while lower doses had little or no effect on the lymphocytotoxin response. A cell-mediated immunity assay showed a substantial response, but one that was lower in amplitude from that of control animals. Histological study of 7th day allograft biopsies demonstrated essentially normal kidneys, except for a mild mononuclear cell infiltrate, at higher doses of cyclosporin. Lower doses of cyclosporin gave a picture of rejection no different from that seen in untreated controls. The LD50 of cyclosporin was found to lie between 50 and 100 mg/kg/day orally. Even the higher of these doses did not cause nephrotoxicity as determined biochemically and histologically.

Published

1980

9. THE DETAILED DISTRIBUTION OF HLA-A, B, C ANTIGENS IN NORMAL HUMAN ORGANS

Author

Fabre Jw, A. Ting, Peter J. Morris, Susan V. Fuggle, and A S Daar

Subjects

Adult, Male, Pathology, medicine.medical_specialty, medicine.drug_class, Respiratory System, Enteroendocrine cell, HLA-C Antigens, Biology, Kidney, Monoclonal antibody, Cardiovascular System, Nervous System, Antigen, HLA Antigens, Endocrine Glands, Testis, medicine, Gastric mucosa, Humans, Transplantation, HLA-A Antigens, Thyroid, Epididymis, HLA-A, medicine.anatomical_structure, HLA-B Antigens, Immunology, Pancreas, Digestive System

Abstract

We have used a monoclonal antibody, PA2.6, directed against the heavy chain of HLA-ABC antigens to study the detailed tissue distribution of MHC class I antigens. Normal tissues from throughout the human body were obtained fresh from organ donors or operative specimens and were snap-frozen in liquid nitrogen within 1-2 hr of removal. Frozen sections were then studied using a sensitive peroxidase-antiperoxidase immunohistological technique. The results of our study show that class I antigens could be detected on most, but not all, the nucleated cells in the body. They were only weakly detectable in several tissues including endocrine cells in the thyroid, parathyroid, pituitary and islets of Langerhans in the pancreas and on gastric mucosa, the myocardium, skeletal muscle, and hepatocytes in some of the specimens. Spermatozoa were positively stained in the testis, but as they moved up into the epididymis class I antigens were no longer detectable. We found that class I antigens were not detectable on corneal endothelium, some Brunner's glands in the duodenum, villous trophoblast, central nervous system neurones, the exocrine portion of the pancreas, and acinar cells in the parotid. We conclude, therefore, that class I antigens are not ubiquitous, as previously thought.

Published

1984

10. LOCALIZATION OF HLA-ABC AND DR ANTIGENS IN HUMAN KIDNEY

Author

Peter J. Morris, Fabre Jw, D. N. J. Hart, Keryn A. Williams, A. Ting, and Susan V. Fuggle

Subjects

Kidney Cortex, medicine.drug_class, Kidney Glomerulus, Biology, Kidney, Monoclonal antibody, Immunofluorescence, Major histocompatibility complex, Antibodies, Mice, Antigen, HLA Antigens, medicine, Animals, Humans, Endothelium, Transplantation, medicine.diagnostic_test, Immunoperoxidase Techniques, Histocompatibility Antigens Class II, Antibodies, Monoclonal, Human kidney, Molecular biology, Kidney Tubules, Immunology, biology.protein, Rabbits

Abstract

Monoclonal antibodies to human monomorphic class I and class II major histocompatibility complex (MHC) determinants have been used with immunofluorescence and immunoperoxidase techniques, to localize these antigens in normal human kidneys. HLA-DR antigen was located in the glomeruli (probably on endothelium as well as the mesangium) and within the cells of cortical and medullary tubules. Dendritic cells in the renal interstitium stained brightly for the DR antigen and could be distinguished from the staining of capillary endothelium. The vascular endothelium of large vessels stained less densely for the HLA-DR antigen than for HLA-ABC antigens. The glomeruli stained intensely for the HLA-ABC antigens and diffuse staining of HLA-ABC antigens was also noted within renal tubular cells.

Published

1981

11. PASSIVE ENHANCEMENT AND HYPERACUTE REJECTION OF RENAL ALLOGRAFTS IN THE RAT

Author

Peter R. Millard, Peter J. Morris, D. N. J. Hart, Fabre Jw, and C. G. Winearls

Subjects

Graft Rejection, Transplantation, Pathology, medicine.medical_specialty, Erythrocytes, business.industry, Rats, Inbred Strains, Kidney Transplantation, Antibodies, Absorption, Rats, Guinea pig, Immunoglobulin Fab Fragments, Red blood cell, medicine.anatomical_structure, Graft Enhancement, Immunologic, HyperAcute Renal, Rats, Inbred Lew, Allograft rejection, medicine, Animals, Transplantation, Homologous, business, Cytotoxic antibody

Abstract

Attempts to induce passive enhancement of renal allografts with donor-specific cytotoxic antibody can result in antibody-mediated damage to the grafted organ. Hyperacute renal allograft rejection occurred in the homozygous DA to Lewis strain combination when Lewis anti-DA serum was administered with guinea pig complement. Hyperacute rejection was prevented in four of five rats when Lewis anti-DA F(ab')2 was injected before the administration of Lewis anti-DA serum and complement and these grafts had enhanced survival. Red blood cell absorption of the Lewis anti-DA serum to produce an anti-Ia-like serum, also removed its ability to produce hyperacute rejection without removing its ability to enhance. With appropriate modifications both of these techniques would be applicable to human transplantation.

Published

1980

12. DISTRIBUTION AND QUANTITATION OF HLA-ABC AND DR (Ia) ANTIGENS ON HUMAN KIDNEY AND OTHER TISSUES

Author

Fabre Jw, D. N. J. Hart, Keryn A. Williams, and Peter J. Morris

Subjects

Isoantigens, medicine.drug_class, T-Lymphocytes, Cell, Radioimmunoassay, Fluorescent Antibody Technique, Spleen, Kidney, Monoclonal antibody, Antigen, HLA Antigens, medicine, Humans, Distribution (pharmacology), Tissue Distribution, Platelet, Immunosorbent Techniques, Transplantation, Chemistry, Myocardium, medicine.anatomical_structure, Liver, Immunology, Bone marrow

Abstract

A quantitative estimation of the amounts of human Ia (HLA-DR) and HLA-ABC antigen on a variety of human tissues was performed. Monoclonal antibodies to species-common determinants of HLA-DR and HLA-ABC antigens were absorbed quantitatively with tissue homogenates and cell suspensions, and reassayed for residual activity in a radioimmunobinding assay. Kidney was found to carry 90% as much HLA-DR and 14% as much HLA-ABC antigen as spleen, while liver contained 19 and 9% as much, respectively. Small amounts of both antigens were found on heart; brain carried very little HLA-ABC and virtually no DR. Neither HLA-ABC nor DR was found on erythrocytes or reticulocytes. Of interest was our finding that a small subpopulation of thymocytes (10%) was HLA-DR positive. Platelets contained approximately 5% of the amount of HLA-ABC as spleen and undetectable quantities of HLA-DR, as expected. Chronic lymphatic leukemia (CLL) cells were found to carry 10% as much HLA-ABC and 33% as much DR antigen as spleen, while the values for bone marrow were 15 and 2%, respectively.

Published

1980

13. Monoclonal anti lymphocyte antibodies as immunosuppressive reagents for clinical practice

Author

Fabre Jw

Subjects

biology, medicine.drug_class, business.industry, Lymphocyte, General Medicine, Lymphocyte antigen, Monoclonal antibody, Clinical Practice, medicine.anatomical_structure, Monoclonal, Immunology, medicine, biology.protein, Antibody, business

Abstract

SynopsisBy the late 1970s it had become clear that the immunosuppressive effects of conventional anti lymphocyte serum (ALS) were mediated by only a small component of the anti lymphocyte antibodies present. This fact meant that attempts to improve the safety, potency and standardisation of conventional ALS by raising xenosera to single, purified lymphocyte antigens were faced with considerable technical and theoretical problems. Coincidentally and very fortunately, it was at this time that the potential of monoclonal antibodies in the field of ALS were becoming obvious. Their advent has dramatically transformed the situation, from a bleak one with few prospects to one where the early promise of ALS is likely to be realised in the clinic within the next few years. This review looks at why it is that monoclonal antibodies have so changed the situation, and then discusses in detail the optimal properties, in terms of specificity and other characteristics, of immunosuppressive monoclonal antibodies, and finally looks at precisely how they should be used in the clinic.

Published

1982

14. QUANTITATIVE STUDIES ON THE TISSUE DISTRIBUTION OF Ia AND SD ANTIGENS IN THE DA AND LEWIS RAT STRAINS

Author

Hart Dn and Fabre Jw

Subjects

Transplantation, Kidney, biology, Rats, Inbred Strains, Spleen, Major histocompatibility complex, Molecular biology, Rats, Major Histocompatibility Complex, medicine.anatomical_structure, Antigen, Rats, Inbred Lew, Histocompatibility Antigens, Immunology, medicine, biology.protein, Animals, Tissue Distribution, Bone marrow, Antibody, Lymph node, Immunosorbent Techniques

Abstract

The tissue distribution of major histocompatibility complex (MHC) antigens in the DA and Lewis (LEW) strains was studied using LEW anti-DA and DA anti-LEW alloantisera. Quantitative absorption analyses were used with quantitative binding assays for SD and Ia antigens. Initial screening showed that the LEW anti-DA serum contained significant amounts of antibodies against both Ia and SD antigens. On the other hand, the DA anti-LEW serum seemed to be directed almost entirely against Ia antigens, and it was not possible to set up assays for SD antigens in the LEW strain. The most surprising finding was the presence of large amounts of Ia antigen on the kidneys of both the DA and LEW strains, one kidney containing as much Ia antigen as half a spleen. Kidney also contained large amounts of SD antigen. Liver had large amounts of SD, but very little Ia. Heart had only small amounts of both SD and Ia. The relevance of these findings to transplantation of the kidney, liver, and heart are discussed. The other tissues studied were brain, spleen, lymph node, thoracic duct lymphocytes, bone marrow, thymus, RBC, and platelets. The most interesting findings were the presence of relatively large amounts of SD antigens on DA RBC, and small amounts of Ia on the thymus and bone marrow.

Published

1979

15. EXPERIENCE WITH PASSIVE ENHANCEMENT OF RENAL ALLOGRAFTS IN A (DA x LEWIS)F1 TO LEWIS STRAIN COMBINATION

Author

Fabre Jw and Morris Pj

Subjects

Graft Rejection, Transplantation, medicine.medical_specialty, Strain (chemistry), business.industry, Immune Sera, Cytotoxicity Tests, Immunologic, Kidney, Kidney Transplantation, Molecular biology, Rats, Surgery, Lewis Blood Group Antigens, Transplantation Immunology, Histocompatibility, Blood Group Antigens, medicine, Animals, Transplantation, Homologous, Urea, Female, Lymphocytes, Antigens, business, Immunity, Maternally-Acquired

Published

1972

16. PROLONGATION OF CARDIAC XENOGRAFT SURVIVAL IN RATS RECEIVING CYCLOSPORIN A

Author

Peter R. Millard, Keryn A. Williams, William P. Homan, Peter J. Morris, and Fabre Jw

Subjects

Male, Transplantation, Heterologous, Hamster, Cyclosporins, Pharmacology, Peptides, Cyclic, Lymphocytotoxic antibody, Cricetinae, Cyclosporin a, Animals, Medicine, Antilymphocyte Serum, Transplantation, Mesocricetus, biology, business.industry, Myocardium, Graft Survival, Rats, Titer, Close relationship, biology.protein, Heart Transplantation, Female, Antibody, business, Immunosuppressive Agents, Median survival

Abstract

SUMMARY The effect of cyclosporin A was tested in a heterotopic cardiac xenograft model, in which hamster hearts were implanted into LEW rats. Despite the presence of low titers of rat anti-hamster lymphocytotoxic antibodies immediate rejection of the hamster hearts did not occur, suggesting that this model represented a xenogeneic barrier of moderate strength, compatible with the close relationship of the two species. Cyclosporin A, in doses approaching toxic levels of 35 or 50 mg/kg/day for 14 days, prolonged function of the cardiac xenografts for median survival times of 21 and 11 days, respectively, in contrast to the median survival of 2 days in untreated recipients. The lymphocytotoxic antibody response of the LEW rats to the cardiac xenograft was suppressed, even in doses that did not prolong graft survival. Only the dose of 50 mg/kg/day produced any significant alteration in the histological features of rejection in the cardiac xenografts. Although cyclosporin A markedly prolonged survival of cardiac xenografts between these two closely related species, the requirement of virtually toxic levels of the drug for an effect do not suggest that this drug will be of value in transplantation of vascularized organ xenografts.

Published

1981

17. Assessment of Homograft Compatibility

Author

Fabre Jw

Subjects

Pathology, medicine.medical_specialty, Graft rejection, business.industry, Organ Graft, medicine.medical_treatment, Immunology, Medicine, Immunosuppression, Human leukocyte antigen, business, medicine.disease, Kidney transplantation

Published

1976

18. A study of three protocols of blood transfusion before renal transplantaion in the dog

Author

T. G. Denton, Keryn A. Williams, Peter R. Millard, Fabre Jw, T. Sen, Peter J. Morris, Judith S. McKenzie, and Matthew Bishop

Subjects

Transplantation, Kidney, Immunity, Cellular, Blood transfusion, business.industry, medicine.medical_treatment, Azathioprine, Hemagglutination Tests, Kidney Transplantation, medicine.anatomical_structure, Dogs, Immunity, Anesthesia, Prednisolone, Methods, Medicine, Animals, Blood Transfusion, business, Positive crossmatch, Canine model, medicine.drug, Antilymphocyte Serum, Autoantibodies

Abstract

Three protocols of blood transfusion were evaluated in a canine model for (1) the strength and breadth of leukocytotoxin induction, (2) the induction of cell-mediated immunity against the blood donors, (3) haemagglutinin production, and (4) any effect on kidney graft survival. At the end of the transfusion schedule, each dog received a kindey graft and was given azathioprine and prednisolone postoperatively. All dogs were unrelated and blood donors were not used as kidney donors. All three transfusion protocols, comprising i.v. injections of blood twice weekly or every 2 weeks from one or three donors, induced unacceptably strong and broad leukocytotoxins. All transplants performed across a positive crossmatch failed to function. However, where a negative crossmatch was available, the trend of results was that the transfused dogs had better graft survival than nontransfused animals similarly treated with azathioprine and prednisolone. Only one dog produced haemagglutinins. Several animals had positive cell-mediated immunity against the blood donors, but the response was not strong and was frequently not sustained.

Published

1978

19. Use of cyclophosphamide and enhancing serum to suppress renal allograft rejection in the rat

Author

Peter R. Millard, Peter J. Morris, Fabre Jw, and C. G. Winearls

Subjects

Graft Rejection, Male, Transplantation, Kidney, medicine.medical_specialty, Cyclophosphamide, Dose-Response Relationship, Drug, business.industry, Urology, Rat strain, Rats, Inbred Strains, Graft function, Kidney Transplantation, Cyclophosphamide treatment, Rats, medicine.anatomical_structure, Graft Enhancement, Immunologic, medicine, Renal allograft, Animals, Transplantation, Homologous, Graft survival, business, medicine.drug

Abstract

Cyclophosphamide was tested for its interaction with passive enhancement in suppressing the rejection of kidney allografts in the (DA x Lewis)F1 to Lewis rat strain. Dose response studies with cyclophosphamide showed that 10 mg/kg/day for 14 days was necessary for complete suppression of rejection and indefinite graft survival. Doses of 5 and 3.5 mg/kg/day had only a marginal effect on graft function and survival, although the lymphocytotoxin response to the graft was completely or very substantially suppressed by these smaller doses. The use of passive enhancement with cyclophosphamide at the 5- and 3.5-mg/kg/day doses resulted in a favourable interaction with improved graft function and survival. Interestingly, passive enhancement in combination with 5 mg/kg/day of cyclophosphamide resulted in indefinite graft survival only if cyclophosphamide was given for 28 days. If cyclophosphamide was given for 14 days, rejection was suppressed only during the period of cyclophosphamide treatment.

Published

1979

20. Vein allografts for arterial replacement in rats: an immunological and histological study

Author

C. G. Winearls, Peter J. Morris, J. K. McGeachie, F. J. Prendergast, and Fabre Jw

Subjects

Male, Pathology, medicine.medical_specialty, Necrosis, Intimal hyperplasia, Time Factors, medicine.medical_treatment, Veins, Fibrosis, Histocompatibility Antigens, medicine, Cytotoxic T cell, Animals, Transplantation, Homologous, Lymphocytes, Vein, Transplantation, Immunity, Cellular, biology, business.industry, Graft Survival, Immunosuppression, Rats, Inbred Strains, Arteries, medicine.disease, Cytotoxicity Tests, Immunologic, Rats, medicine.anatomical_structure, Phenotype, Rats, Inbred Lew, biology.protein, Iliolumbar Vein, Antibody, medicine.symptom, business

Abstract

Vein allografts were studied in the rat using the major histocompatibility complex-incompatible DA and Lewis inbred strains. Allografts were performed in the Lewis to DA and DA to Lewis combinations, with Lewis to Lewis isografts serving as controls. Vein grafts were performed by interposing a 1 cm length of fresh iliolumbar vein into a defect of the iliac artery, using microsurgical techniques. The grafts were under observation for 18 weeks for (1) patency, (2) gross structural changes, (3) histological changes, and (4) antibody responses. No immunosuppression was used. All grafts remained patient throughout the period of observation, although aneurysm formation was noted in some allografts toward the end of the observation period. Histologically, allografts and isografts were indistinguishable. In the first 2 weeks, they showed patchy areas of necrosis in the vein walls, with subsequent intimal hyperplasia and medial fibrosis. In both strain combinations a lymphocytotoxin response was induced in most animals, the response being particularly strong in the DA to Lewis combination. All cytotoxic activity could be absorbed out using red blood cells, suggesting that the specificity of the antibody was mainly or entirely directed against SD antigens.

Published

1979

21. THE ROLE OF PASSENGER LEUCOCYTES IN THE REJECTION OF RENAL ALLOGRAFTS IN THE RAT

Author

Morris Pj and Fabre Jw

Subjects

Graft Rejection, Isoantigens, Time Factors, Bone Marrow Cells, Text mining, Bone Marrow, Leukocytes, Animals, Transplantation, Homologous, Urea, Medicine, Lymphocytes, Antigens, Cyclophosphamide, Bone Marrow Transplantation, Transplantation, Mosaicism, business.industry, Immune Sera, Cytotoxicity Tests, Immunologic, Kidney Transplantation, Rats, Rats, Inbred Lew, Immunology, Female, business, Spleen

Published

1973

22. In vivo studies on non-viral transdifferentiation of liver cells towards pancreatic β cells.

Author

Cim A, Sawyer GJ, Zhang X, Su H, Collins L, Jones P, Antoniou M, Reynes JP, Lipps HJ, and Fabre JW

Subjects

Animals, Basic Helix-Loop-Helix Transcription Factors genetics, Diabetes Mellitus, Experimental therapy, Homeodomain Proteins genetics, Hyperglycemia therapy, Insulin metabolism, Insulin-Secreting Cells physiology, Liver physiology, Maf Transcription Factors, Large genetics, Male, Nerve Tissue Proteins genetics, Pancreas cytology, Pancreas physiology, Plasmids genetics, Rats, Rats, Inbred Strains, Trans-Activators genetics, Transcription, Genetic genetics, Cell Differentiation genetics, Diabetes Mellitus, Type 1 therapy, Gene Transfer Techniques, Genetic Therapy methods, Insulin-Secreting Cells cytology, Liver cytology

Abstract

Transdifferentiation in vivo is an attractive option for autologous replacement of pancreatic β cells in patients with type 1 diabetes. It has been achieved by adenoviral delivery of genes for transcription factors in the liver and pancreas of hyperglycaemic mice. However, these viral approaches are not clinically applicable. We used the hydrodynamic approach to deliver genes Pdx1, Ngn3 (Neurog3) and MafA singly and in combination to livers of normoglycaemic rats. Five expression plasmids were evaluated. Livers were removed 1, 3, 7, 14 and 28 days after gene delivery and assayed by quantitative PCR, semi-quantitative PCR and immunohistology. Functional studies on hyperglycaemic rats were performed. The highest and most sustained expression was from a CpG-depleted plasmid (pCpG) and a plasmid with an in-frame scaffold/matrix attachment region ((pEPI(CMV)). When Pdx1, Ngn3 and MafA were delivered together to normoglycaemic rats with these plasmids, insulin mRNA was detected at all time points and was ~50-fold higher with pCpG. Insulin mRNA content of livers at days 3 and 7 was equivalent to that of a pancreas, with scattered insulin-positive cells detected by immunohistology, but levels declined thereafter. Prohormone convertase 1/3 was elevated at days 3 and 7. In hyperglycaemic rats, fasting blood glucose was lower at days 1, 3 and 7 but not thereafter, and body weight was maintained to day 28. We conclude that hydrodynamic gene delivery of multiple transcription factors to rat liver can initiate transdifferentiation to pancreatic β cells, but the process is reversible and probably requires more sustained transcription factor expression.

Published

2012

23. Critical physiological and surgical considerations for hydrodynamic pressurization of individual segments of the pig liver.

Author

Fabre JW, Whitehorne M, Grehan A, Sawyer GJ, Zhang X, Davenport M, and Rela M

Subjects

Animals, Blood Pressure, DNA administration & dosage, Female, Fluoroscopy, Gene Expression, Genetic Therapy, Luciferases analysis, Luciferases genetics, Plasmids metabolism, Portal Vein metabolism, Swine, Gene Transfer Techniques, Hydrodynamics, Liver physiology, Liver surgery

Abstract

Hydrodynamic gene delivery to the liver is a promising approach for liver gene therapy in the clinic, but levels of gene expression in larger species have been much less than in rodents. The development of surgical techniques for pressurizing individual liver segments and the establishment of whether hepatic vascular anatomy in fact permits pressurization of individual segments are critical issues that need to be addressed. We have evaluated these issues using hydrodynamic delivery to individual segments of the pig liver, via branches of both portal and hepatic veins. Our objective was to develop surgical techniques that achieve elevated vascular pressures within individual liver segments with small volumes, but without interruption of portal blood flow or reduction in venous return to the heart. We report that, without specific surgical interventions to obstruct outflow of DNA solution from the targeted liver segment, little or no increase in intrahepatic vascular pressure occurs. We demonstrate, for the first time, that selective pressurization of individual liver segments is possible without compromising portal venous flow or venous return to the heart. Thus, hydrodynamic gene delivery to individual liver segments is technically achievable in a clinical setting, but will require open abdominal surgery rather than minimally invasive techniques.

Published

2011

24. Self-assembly of peptides into spherical nanoparticles for delivery of hydrophilic moieties to the cytosol.

Author

Collins L, Parker AL, Gehman JD, Eckley L, Perugini MA, Separovic F, and Fabre JW

Subjects

Amino Acid Sequence, Cell Line, Hydrophobic and Hydrophilic Interactions, Models, Molecular, Molecular Imaging, Molecular Sequence Data, Particle Size, Protein Binding, Protein Conformation, Cytosol metabolism, Endocytosis, Nanoparticles chemistry, Peptides chemistry, Peptides metabolism

Abstract

We report a novel class of self-assembling peptide nanoparticles formed by mixing aqueous solutions of K(16) peptide and a 20 amino acid peptide of net charge -5 (GLFEALLELLESLWELLLEA). Particle formation is salt-dependent and yields perfectly spherical nanoparticles of approximately 120 to approximately 800 nm diameter, depending on buffer composition and temperature, with a stoichiometry of approximately 1:2.5 for the cationic and anionic peptides. The anionic peptide forms an alpha-helix in aqueous solution, has all five glutamates on one side of the helix, and exists entirely as a discrete oligomer of 9-10 peptides. A rigid oligomer with 45-50 negative charges almost certainly represents the core component of these nanoparticles, held together by electrostatic interactions with the unstructured K(16) peptide. Cells internalize these particles by an endocytic process, and free particles are frequently seen in the cytosol, presumably because of the acid-dependent fusogenic properties of the anionic peptide. Among other applications, these particles have potential for the targeted delivery of single or multiple therapeutic moieties directly to the cytosol, and we report the successful delivery of a K(16)-linked pro-apoptosis peptide.

Published

2010

25. Technical requirements for effective regional hydrodynamic gene delivery to the left lateral lobe of the rat liver.

Author

Sawyer GJ, Zhang X, and Fabre JW

Subjects

Animals, Liver metabolism, Rats, Gene Transfer Techniques, Genetic Therapy methods, Liver surgery

Abstract

Hydrodynamic gene delivery to the liver is an attractive approach for clinical liver gene therapy, but critical aspects of technique remain uncertain. There has not been to date any report of high levels of hydrodynamic gene delivery to the liver, except in rodents. Regional hydrodynamic delivery to individual lobes/segments of the liver is being pursued in preclinical pig models, where reporter gene expression has been <1% of rodent levels, and in one clinical study, where there was no substantive evidence of gene expression. In none of these studies did surgical technique include outflow obstruction of the DNA solution. Here we report a novel technique for regional hydrodynamic gene delivery to the left lateral lobe of the rat liver. The technique gives high levels of gene delivery specific to the left lateral lobe with low volumes ( approximately 1.5 ml) of DNA solution, and permits an evaluation of hydrodynamic delivery in the presence and in the absence of outflow obstruction. We report that outflow obstruction is an absolute requirement for effective hydrodynamic gene delivery to individual lobes/segments of the liver, and therefore that minimally invasive techniques will not be possible in the clinic.

Published

2010

26. Hydrodynamic gene delivery to the liver: theoretical and practical issues for clinical application.

Author

Sawyer GJ, Rela M, Davenport M, Whitehorne M, Zhang X, and Fabre JW

Subjects

Animals, Genetic Vectors genetics, Humans, Models, Animal, Transduction, Genetic, Genetic Therapy methods, Liver metabolism

Abstract

Hydrodynamic gene delivery to the liver has potential as a safe and effective approach for clinical liver gene therapy. However, the simplicity of the technique in rodents - an intravenous injection - belies the theoretical and practical complexity for clinical application. A key issue is that outflow obstruction of the DNA solution from the liver is a critical factor for raising intrahepatic vascular pressure, which in turn provides the force to swell the liver and effect gene delivery. For conventional hydrodynamic gene delivery via tail vein injection, this outflow obstruction is provided naturally by the vascular resistance of the gut, spleen and pancreas. For regional hydrodynamic gene delivery to the liver, outflow obstruction to create a closed system requires surgical intervention, making it unlikely that minimally invasive techniques will be possible in the clinic. Intrinsic factors, in particular compliance (elasticity) of the liver are likely to be crucial in determining the degree of swelling for a given level of intrahepatic vascular pressure. Liver compliance is likely to be the major reason for the low level of hydrodynamic gene delivery in the pig model, and will influence the effectiveness of the approach in man, both in general and in different disease states.

Published

2009

27. Intestinal lactase as an autologous beta-galactosidase reporter gene for in vivo gene expression studies.

Author

Salehi S, Eckley L, Sawyer GJ, Zhang X, Dong X, Freund JN, and Fabre JW

Subjects

Animals, Cell Line, Tumor, Gene Transfer Techniques, Humans, Lactase administration & dosage, Lactase genetics, Liver metabolism, Mice, Promoter Regions, Genetic, Rats, Transfection, beta-Galactosidase metabolism, Gene Expression, Genes, Reporter, Intestinal Mucosa metabolism, Lactase metabolism, beta-Galactosidase genetics

Abstract

Intestinal lactase has potential as an autologous beta-galactosidase reporter gene for long-term gene expression studies in vivo, using chromogenic, luminescent, and fluorogenic substrates developed for Escherichia coli beta-galactosidase. In normal rat tissues, reactivity with a chromogenic fucopyranoside (X-Fuc, the preferred substrate of lactase) was present only at the lumenal surface of small intestine epithelial cells. Full-length lactase (domains I-IV), mature lactase (domains III and IV), and a cytosolic form of mature lactase (domains III and IV, without the signal sequence or transmembrane region) were evaluated. Transfection of HuH-7 cells in vitro, and hydrodynamic gene delivery to the liver in vivo, resulted in excellent gene expression. The full-length and mature (homodimeric, membrane-bound) forms reacted strongly with X-Fuc but not with the corresponding galactopyranoside (X-Gal). However, the presumptively monomeric cytosolic lactase unexpectedly reacted equally well with both substrates. The fluorogenic substrate fluorescein-di-beta-D-galactopyranoside was cleaved by cytosolic lactase, but not by full-length or mature lactase. Full-length lactase, when expressed ectopically in hepatocytes in vivo, localized exclusively to the bile canalicular membrane. Intestinal lactase is highly homologous in mice, rats, and humans and has considerable potential for evaluating long-term gene expression in experimental animals and the clinic.

Published

2009

28. Low-volume hydrodynamic gene delivery to the rat liver via an isolated segment of the inferior vena cava: efficiency, cardiovascular response and intrahepatic vascular dynamics.

Author

Sawyer GJ, Grehan A, Dong X, Whitehorne M, Seddon M, Shah AM, Zhang X, Salehi S, and Fabre JW

Subjects

Animals, Blood Pressure, Electrocardiography, Genetic Therapy adverse effects, Heart Rate, Infusions, Intravenous adverse effects, Infusions, Intravenous methods, Liver blood supply, Male, Rats, Rats, Inbred Strains, Cardiovascular Physiological Phenomena drug effects, DNA administration & dosage, Genetic Therapy methods, Liver metabolism, Vena Cava, Inferior

Abstract

Background: Clinical application of hydrodynamic gene delivery to the liver requires the use of small volumes, an evaluation of the cardiovascular consequences of acute volume overload, and a better understanding of the intrahepatic vascular pressures driving gene delivery. Injection of DNA solution into the isolated segment of inferior vena cava (IVC) draining the hepatic veins is a potentially valuable low-volume approach., Methods: Various volumes of DNA solution (pGL3 plasmid) were injected at 100 ml/min either systemically or into the isolated IVC segment in the DA rat. Arterial pressure, portal venous pressure, heart rate and electrocardiogram, in addition to reporter gene expression in the liver, were monitored., Results: The 2% volume was > 10 000-fold more effective when delivered via the IVC segment than when given systemically, and as effective as 6% systemically. Isolation of the IVC segment caused profound falls in arterial pressure, with electrocardiogram signs of myocardial ischemia. On release of the IVC ties, without DNA infusion (no volume overload), arterial pressure recovered rapidly. However, with DNA infusion (volume overload) there was a brief recovery of arterial pressure, followed by complete heart block and fall in arterial pressure and pulse for several minutes. Portal venous pressure rose steeply to 30-33 mm Hg during the infusion., Conclusions: The IVC segment approach enables excellent gene delivery to the whole liver with small volumes, but causes severe cardiovascular disturbances in the rat. Portal venous pressures are slightly higher than in the mouse, and suggest functional outflow obstruction by the capillary bed of the intestines.

Published

2008

29. Hydrodynamic gene delivery to the pig liver via an isolated segment of the inferior vena cava.

Author

Fabre JW, Grehan A, Whitehorne M, Sawyer GJ, Dong X, Salehi S, Eckley L, Zhang X, Seddon M, Shah AM, Davenport M, and Rela M

Subjects

Animals, Cell Line, Female, Fluoroscopy, Gene Expression, Liver metabolism, Luciferases genetics, Models, Animal, Rats, Rats, Inbred Strains, Swine, Venous Pressure, DNA administration & dosage, Gene Transfer Techniques, Genetic Therapy methods, Liver Diseases therapy, Vena Cava, Inferior

Abstract

Hydrodynamic gene delivery is an attractive option for non-viral liver gene therapy, but requires evaluation of efficacy, safety and clinically applicable techniques in large animal models. We have evaluated retrograde delivery of DNA to the whole liver via the isolated segment of inferior vena cava (IVC) draining the hepatic veins. Pigs (18-20 kg weight) were given the pGL3 plasmid via two programmable syringe pumps in parallel. Volumes corresponding to 2% of body weight (360-400 ml) were delivered at 100 ml s(-1) via a Y connector. The IVC segment pressure, portal venous pressure, arterial pressure, electrocardiogram (ECG) and pulse were monitored. Concurrent studies were performed in rats for interspecies comparisons. The hydrodynamic procedure generated intrahepatic vascular pressures of 101-126 mm Hg, which is approximately 4 times higher than in rodents, but levels of gene delivery were approximately 200-fold lower. Suprahepatic IVC clamping caused a fall in arterial pressure, with the development of ECG signs of myocardial ischaemia, but these abnormalities resolved rapidly. The IVC segment approach is a clinically acceptable approach to liver gene therapy. However, it is less effective in pigs than in rodents, possibly because of larger liver size or a less compliant connective tissue framework.

Published

2008

30. (LYS)(16)-based reducible polycations provide stable polyplexes with anionic fusogenic peptides and efficient gene delivery to post mitotic cells.

Author

Parker AL, Eckley L, Singh S, Preece JA, Collins L, and Fabre JW

Subjects

Adenoviridae, Animals, Cell Line, Cornea cytology, HeLa Cells, Humans, Male, Membrane Fusion, Nanoparticles, Polyelectrolytes, Rabbits, Resting Phase, Cell Cycle, Gene Transfer Techniques, Genetic Vectors, Peptides administration & dosage, Polyamines administration & dosage, Polylysine administration & dosage

Abstract

Extracellular stability, endocytic escape, intracellular DNA release and nuclear translocation of DNA are all critical properties of non-viral vector/DNA particles. We have evaluated a (Lys)(16)-based linear, reducible polycation (RPC) in combination with an acid-dependent, anionic fusogenic peptide for gene delivery to dividing and post-mitotic cells. The RPC was formed from Cys(Lys)(16)Cys monomers. Molecular weight was 24,000 Da, corresponding to an average of 10.5 peptide monomers per RPC. Non-reducible polylysine (PLL) (27,000 Da) and monomeric (Lys)(16) peptide were evaluated for comparison. (Lys)(16)/DNA particles were disrupted at fusogenic peptide concentrations well below those used for gene delivery. By contrast, RPC/DNA an PLL/DNA particles were stable in the presence of high concentrations of the anionic peptide. Addition of 10% serum virtually abolished the transfection ability of (Lys)(16)/DNA/fusogenic peptide particles, but had little effect on RPC/DNA/fusogenic peptide particles. RPC/DNA/fusogenic peptide particles were highly effective for gene delivery to both cell lines and post-mitotic corneal endothelium. PLL/DNA/fusogenic peptide particles were moderately effective on cell lines, but gave no gene delivery with corneal endothelial cells. We conclude that (Lys)(16)-based RPC/DNA/fusogenic peptide particles provide a gene delivery system which is potentially stable in the extracellular environment and, on reductive depolymerisation, can release DNA plasmids for nuclear translocation.

Published

2007

31. Cardiovascular function following acute volume overload for hydrodynamic gene delivery to the liver.

Author

Sawyer GJ, Dong X, Whitehorne M, Grehan A, Seddon M, Shah AM, Zhang X, and Fabre JW

Subjects

Animals, Aorta, Atropine administration & dosage, Blood Pressure, Central Venous Pressure, Electrocardiography, Infusions, Intra-Arterial, Isotonic Solutions, Liver pathology, Luciferases genetics, Male, Parasympatholytics administration & dosage, Pulse, Rats, Rats, Inbred Strains, Ringer's Solution, Signal Processing, Computer-Assisted, Vena Cava, Inferior, Video Recording, Cardiovascular Physiological Phenomena, DNA administration & dosage, Genetic Therapy adverse effects, Genetic Therapy methods, Liver enzymology

Abstract

Hydrodynamic gene delivery to the liver is a valuable experimental tool and an attractive option for nonviral gene therapy of liver disease. However, little attention has been paid to the major obstacle to clinical application: acute volume overload of the cardiovascular system. We delivered volumes of DNA solution (pGL3 plasmid) corresponding to 1, 2, 4, 6 and 8% of the body weight at 100 ml/min to the inferior vena cava (IVC) of DA strain rats. Central venous pressure (CVP), arterial pressure, pulse and electrocardiogram (ECG) were continuously recorded for subsequent analysis. Each volume produced a characteristic response, but all (including the 1% volume) caused severe falls in blood pressure and pulse within 1-2 s of the infusion, with ectopic beats and widening of the QRS complex in the ECG. The response to volumes of 4% and higher suggested that the liver acted as a volume sink, mitigating the immediate effects of volume overload. The 6 and 8% volumes caused profound and protracted falls in blood pressure and pulse, with a multitude of severe electrical abnormalities in the heart, including electromechanical dissociation. Vagal blockade with atropine, and the use of Ringer's solution to prevent electrolyte disturbances, did not ameliorate this picture.

Published

2007

32. Pancreatic duodenal homeobox 1 expression is insufficient to transdifferentiate liver cells into insulin-secreting cells.

Author

Wu Y, Minger SL, Sawyer GJ, Fabre JW, Persaud SJ, and Jones PM

Subjects

Animals, Cell Differentiation physiology, Cloning, Molecular, Hepatocytes metabolism, Humans, Insulin metabolism, Insulin Secretion, Diabetes Mellitus, Type 1 therapy, Hepatocytes cytology, Homeodomain Proteins physiology, Tissue Engineering methods, Trans-Activators physiology

Published

2007

33. Preliminary evidence that the allogeneic response might trigger antitumour immunity in patients with advanced prostate cancer.

Author

Muir G, Rajbabu K, Callen C, and Fabre JW

Subjects

Aged, Aged, 80 and over, Humans, Male, Middle Aged, Prostate-Specific Antigen blood, Prostatic Neoplasms immunology, Transplantation, Autologous, Treatment Outcome, Immunotherapy methods, Lymphocyte Activation immunology, Prostate-Specific Antigen immunology, Prostatic Neoplasms therapy, Skin Transplantation immunology, T-Lymphocytes immunology

Abstract

Objective: To explore the possibility that allogeneic responses might, by chance, encompass cross-reactive T cell clones specific for neo-antigenic tumour determinants, and thereby activate antitumour immunity; such cross-reactions are well documented for antiviral immunity, and genetic instability in developing cancers generates many neo-antigenic determinants as potential targets for immune responses, but the biology inevitably favours tumour progression., Patients and Methods: Fourteen patients with hormone-refractory prostate cancer received full-thickness skin allografts from different, unrelated donors (fellow patients) until each had received six grafts. Serum prostate-specific antigen (PSA) level was used as a surrogate for tumour mass., Results: One patient had a remarkable decline in PSA level, with levels at 1 year lower than before grafting. A second patient had stable PSA levels for almost 2 years. A third patient had stable PSA levels for 10-12 months before they resumed an exponential rise. Of four patients with PSA levels of > 10 ng/mL, three required surgery or radiotherapy for obstructive symptoms during or shortly after grafting., Conclusion: Transplant rejection involves mechanistically atypical T cell recognition of allogeneic major histocompatibility complex antigens, with massive polyclonal T cell activation. This unique aspect of T cell biology might represent a novel approach for initiating cross-reactive antitumour responses.

Published

2006

34. Synthetic peptides as non-viral DNA vectors.

Author

Fabre JW and Collins L

Subjects

Amino Acid Sequence, Animals, Humans, Molecular Sequence Data, Gene Targeting, Genetic Therapy, Genetic Vectors, Peptides

Abstract

The use of multiple peptide motifs to provide effective gene delivery holds great promise as an elegant, non-immunogenic approach to gene therapy. The molecular understanding of cell and viral biology provides a strong foundation on which to pursue this objective. Synthetic peptides containing multiple lysines and/or arginines (occasionally ornithines) provide natural polycations for multivalent electrostatic binding of DNA, and for DNA compaction into particles suitable for gene delivery. These cationic peptides can incorporate additional functional motifs (e.g. for translocating DNA into the nucleus) and they can be linked by disulphide bonds to produce high molecular reducible polycations with superior properties for gene therapy. Many factors influence the size, surface charge and stability of peptide/DNA particles. For in vivo use, uncharged particles resistant to disruption by salt and protein, and targeted to tissue-specific membrane molecules, will be required. Entry into the cell is via one of the endocytic pathways, depending on particle size and (in principle) the target cell surface molecule. Peptide motifs for endocytic escape are based mainly on the anionic fusogenic peptide of influenza virus haemagglutinin and on histidine-rich peptides (where the buffering properties of the imidazole group cause osmotic swelling and probably rupture of endocytic vesicles). Once in the cytosol, translocation of DNA plasmids across the nuclear pore complex into the nucleus is a crucial step, because most target cells for gene therapy are either non-dividing or slowly dividing. Nuclear translocation can be achieved by classical nuclear localising motifs, or more simply by (Lys)16 and other cationic peptides.

Published

2006

35. In vivo suppression of major histocompatibility complex class II expression on porcine vascular endothelial cells by an HMG-CoA reductase inhibitor.

Author

Geissler I, Collins L, Schofield R, and Fabre JW

Subjects

Animals, Atorvastatin, Endothelial Cells immunology, Fluorescent Antibody Technique, Immunoenzyme Techniques, Male, Swine, Endothelial Cells drug effects, Heptanoic Acids pharmacology, Histocompatibility Antigens Class II analysis, Hydroxymethylglutaryl-CoA Reductase Inhibitors pharmacology, Pyrroles pharmacology

Abstract

Background: Vascular endothelial cells of man and pig, but not rodents, strongly express major histocompatibility complex (MHC) class II antigens in vivo, probably via the inducible promoter IV of the class II transactivator. There is abundant in vitro evidence that MHC class II positive vascular endothelial cells can activate T cells. Peripheral antigen presentation by endothelial cells is potentially important for organ-specific immunity, for allograft rejection, and possibly for immune responsiveness in general. Given the reported effects of statins on promoter IV of the class II transactivator, we evaluated in vivo expression of MHC class II antigens in pigs treated with atorvastatin calcium., Methods: Pigs were given 3 mg/kg/day of atorvastatin orally daily for 16 days, and then killed 24 hr after the last dose. Heart, kidney, and liver were removed for immunohistological and quantitative absorption analysis., Results: Double-labeling studies using immunofluorescence on frozen section for Factor VIII and MHC class II showed a marked suppression of MHC class II on vascular endothelial cells in all 4 treated pigs, in comparison with untreated pigs. This was confirmed using immunoperoxidase techniques on frozen sections. Quantitative absorption analysis showed up to 25-fold reduction in MHC class II expression., Conclusions: Statins substantially suppress endothelial cell MHC class II expression in vivo. This is likely to inhibit organ-specific immune responses, and possibly also general immune responsiveness. In a transplantation setting, in addition to other regulatory effects on the recipients immune system, statins might reduce the long-term capacity of the donor organ to activate rejection mechanisms.

Published

2006

36. The effect of anti-lymphocyte serum on subpopulations of blood and tissue leucocytes: possible supplementary mechanisms for suppression of rejection and the development of opportunistic infections.

Author

Geissler I, Sawyer GJ, Dong X, Kandil H, Davies ET, and Fabre JW

Subjects

Animals, Antibodies, Monoclonal chemistry, Blood Cell Count, Cell Separation, Dendritic Cells cytology, Dendritic Cells metabolism, Flow Cytometry, Heart Transplantation adverse effects, Heart Transplantation methods, Immunohistochemistry, Immunosuppressive Agents pharmacology, Killer Cells, Natural metabolism, Leukocytes cytology, Leukocytes metabolism, Macrophages metabolism, Male, Microscopy, Fluorescence, Monocytes metabolism, Opportunistic Infections prevention & control, Rabbits, Rats, Rats, Inbred Lew, Species Specificity, Time Factors, Treatment Outcome, Antilymphocyte Serum therapeutic use

Abstract

Xenogeneic anti-lymphocyte serum (ALS) remains a major reagent for immunosuppression in clinical practice, but mechanisms of action and risks of opportunistic infection have not been considered in the context of innate immunity and its role in immune responsiveness. Rabbit anti rat ALS was administered intraperitoneally. Blood was taken for flow cytometry to establish absolute counts of leucocyte subsets. Tissues were harvested for immunohistology to evaluate interstitial dendritic cells and tissue macrophages. At day 2 of ALS therapy, T cells are completely depleted, as anticipated. B cells are undiminished and form approximately 90% of blood leucocytes. Monocytes and natural killer (NK) cells are substantially (approximately 80%), but not completely, depleted, and there is a trend for diminished numbers of putative dendritic cells. Neither interstitial dendritic cells nor tissue macrophages in heart are affected. The results at day 7 were very similar to day 2. Substantial depletion of blood monocytes and NK cells might attenuate the innate immune system, and represent a possible supplementary mechanism (in addition to T cell depletion) for suppression of rejection. It might be of particular importance in reducing defences against infections. Monitoring these parameters could be of clinical value.

Published

2005

37. Exploration of peptide motifs for potent non-viral gene delivery highly selective for dividing cells.

Author

Parker AL, Collins L, Zhang X, and Fabre JW

Subjects

Adenoviridae, Animals, Biological Transport physiology, Cell Line, Tumor, Cell Survival, Circular Dichroism, Electrophoresis, Agar Gel, Endothelium, Corneal metabolism, Genetic Vectors therapeutic use, Humans, Luciferases, Nanostructures, Particle Size, Plasmids genetics, Plasmids physiology, Protein Conformation, Rabbits, Transfection methods, Amino Acid Motifs genetics, Genetic Therapy methods, Genetic Vectors genetics, Lipids chemistry, Peptides genetics, Peptides metabolism, Polyethyleneimine metabolism

Abstract

Background: The immunogenicity of viral DNA vectors is an important problem for gene therapy. The use of peptide motifs for gene delivery would largely overcome this problem, and provide a simple, safe and powerful approach for non-viral gene therapy., Methods: We explored the functional properties of two motifs: the (Lys)(16) motif (for binding and condensing DNA, and probably also nuclear translocation of plasmids) and the fusogenic peptide motif of influenza virus (for acid-dependent endocytic escape of peptide/DNA particles). The physical properties and gene delivery efficiencies of (Lys)(16)-containing peptides in combination with free fusogenic peptide were evaluated, and compared with a single composite peptide incorporating both moieties. Post-mitotic corneal endothelial cells and growth-arrested HeLa were included, so as not to neglect the question of nuclear translocation of plasmids., Results: The fusogenic moiety in the composite peptide was able to adopt an alpha-helical configuration unhindered by the (Lys)(16) moiety, and retained acid-dependent fusogenic properties. The composite peptide gave remarkably high levels of gene delivery to dividing cell lines. However, in marked contrast to (Lys)(16)/DNA complexes plus free fusogenic peptide, the composite peptide was completely ineffective for gene delivery to post-mitotic and growth-arrested cells., Conclusions: Attachment of the fusogenic peptide to (Lys)(16) appears to block (Lys)(16)-mediated nuclear translocation of plasmid, but not fusogenic peptide mediated endocytic escape. This strengthens the experimental basis for (Lys)(16)-mediated nuclear translocation of plasmids, and provides a single peptide with potent gene delivery properties, restricted to dividing cells. This property is potentially useful in experimental biology and clinical medicine.

Published

2005

38. A remarkable permeability of canalicular tight junctions might facilitate retrograde, non-viral gene delivery to the liver via the bile duct.

Author

Hu J, Zhang X, Dong X, Collins L, Sawyer GJ, and Fabre JW

Subjects

Animals, Cell Line, Chelating Agents pharmacology, Egtazic Acid pharmacology, Gene Expression, Gold administration & dosage, Infusions, Parenteral methods, Lysine genetics, Nanostructures, Oligopeptides genetics, Particle Size, Permeability, Rats, Rats, Inbred Lew, Bile Canaliculi, Gene Transfer Techniques, Liver drug effects, Liver ultrastructure, Tight Junctions physiology

Abstract

Aims: To establish the extent of retrograde bile duct infusion at an ultrastructural level, as a preliminary step before evaluating the efficacy of gene delivery to the rat liver via a branch of the bile duct., Methods: The extent of retrograde infusion into the biliary tree was established by light and electron microscopy, following infusion of 10 nm gold particles into the right lateral lobe. Canalicular permeability was further assessed by the infusion of a 67 kDa protein. For gene delivery, both naked DNA and a synthetic peptide vector system were evaluated. Because canalicular tight junction permeability can be compromised in damaged livers, both normal rats and rats recovering from the hepatotoxin D-galactosamine were studied., Results: The gold particles penetrated the peripheral one third of the hepatic lobules and, surprisingly, reached the space of Disse in normal rats. Equally surprisingly, blood levels of a 67 kDa protein were identical after bile duct infusion and portal vein injection. Gene delivery with peptide/DNA complexes was much more effective in rats treated with D-galactosamine. However, gene delivery with naked DNA was equally effective in normal and damaged livers. Localisation of gene expression showed a scattering of positive hepatocytes restricted to the right lateral lobe., Conclusions: Retrograde infusion into the bile duct advances well into the hepatic lobule and reveals a remarkable permeability of the canalicular or cholangiole tight junctions in normal rats. It is an effective approach for delivering genes to a small population (approximately 1%) of hepatocytes.

Published

2005

39. Regional hydrodynamic gene delivery to the rat liver with physiological volumes of DNA solution.

Author

Zhang X, Dong X, Sawyer GJ, Collins L, and Fabre JW

Subjects

Amino Acid Sequence, Animals, Chloroquine pharmacology, DNA chemistry, Endocytosis drug effects, Gene Expression, Genetic Vectors administration & dosage, Isotonic Solutions administration & dosage, Liver pathology, Liver physiology, Luciferases genetics, Molecular Sequence Data, Portal Vein, Rats, Rats, Inbred Strains, Tissue Distribution, Vena Cava, Inferior, DNA administration & dosage, Gene Transfer Techniques, Liver drug effects

Abstract

Background: The major barrier to the clinical application of hydrodynamic gene delivery to the liver is the large volume of fluid required using standard protocols. Regional hydrodynamic gene delivery via branches of the portal vein has not previously been reported, and we have evaluated this approach in a rat model., Methods: The pGL3 plasmid with the luciferase reporter gene was used at 50 micro g/ml in isotonic solutions, and was administered with a syringe pump for precise control of the hydrodynamic conditions evaluated. Gene expression was individually measured in six anatomically distinct liver lobes. The effect of systemic chloroquine to promote endocytic escape and a (Lys)(16)-containing peptide to condense the DNA into approximately 100-nm nanoparticles was also evaluated., Results: Hydrodynamic conditions for excellent gene delivery were obtained by using 3-ml volumes ( approximately 12 ml/kg) of isotonic DNA solution delivered at 24 ml/min to the right lateral lobe ( approximately 20% of the liver mass). Under these conditions, >95% of gene delivery usually occurred in the targeted right lateral lobe. Outflow obstruction was essential for gene delivery, both at optimal and at very low levels of hydrodynamic gene delivery. The use of systemic chloroquine to promote endocytic escape did not augment hydrodynamic gene delivery, while condensation of DNA in non-ionic isotonic solutions (5% dextrose) to nanoparticles of approximately 100 nm completely abolished gene delivery., Conclusions: Regional hydrodynamic gene delivery via a branch of the portal vein offers a physiological model of liver gene therapy, for experimental and clinical application., (Copyright 2004 John Wiley & Sons, Ltd.)

Published

2004

40. Imaging in solution of (Lys)(16)-containing bifunctional synthetic peptide/DNA nanoparticles for gene delivery.

Author

Collins L, Kaszuba M, and Fabre JW

Subjects

Carrier Proteins chemistry, Carrier Proteins metabolism, Crotalid Venoms chemistry, Crotalid Venoms metabolism, DNA metabolism, Gene Transfer Techniques, Genetic Vectors metabolism, Integrins metabolism, Peptide Fragments chemistry, Peptide Fragments metabolism, Polylysine metabolism, DNA chemistry, Genetic Vectors chemistry, Polylysine chemistry

Abstract

The physical properties of non-viral vector/DNA nanoparticles in physiological aqueous solution are poorly understood. A Fluid Particle Image Analyser (FPIA), normally used for analysis of industrial and environmental fluids, was used to visualise individual (Lys)(16)-containing peptide/DNA particles. Eight (Lys)(16)-containing synthetic peptides were used to generate peptide/DNA particles at a constant + to - charge ratio of 2.8:1 with 10 microg/ml of plasmid DNA in phosphate buffered saline. Dynamic Light Scattering (DLS) and gene delivery studies were also performed. We present the first images of non-viral vector/DNA nanoparticles in physiological aqueous solution, together with precise measurements of individual particle size and shape in solution and, for the first time, an accurate measure of particle number. Particle size and shape, particle number, and efficiency for gene delivery varied markedly with different peptides. Under standard conditions for in vitro gene delivery, we estimate approximately 60 peptide/DNA nanoparticles per target cell, each containing approximately 70,000 plasmids. This novel capacity to image individual vector/DNA nanoparticles in solution and to count them accurately will enable a more precise assessment of non-viral gene delivery systems, and a more quantitative interpretation of gene delivery experiments.

Published

2004

41. A synthetic peptide vector system for optimal gene delivery to corneal endothelium.

Author

Collins L and Fabre JW

Subjects

Animals, Carrier Proteins metabolism, Crotalid Venoms metabolism, DNA metabolism, Endothelium metabolism, Genes, Reporter, Male, Mitosis physiology, Peptide Fragments metabolism, Rabbits, Time Factors, Cornea metabolism, Gene Transfer Techniques, Genetic Vectors, Peptides

Abstract

Background: Efficient and non-toxic gene delivery, preferably with non-viral DNA vectors readily transferable to clinical practice, is generally regarded as a major limitation for gene therapy., Methods: A 31 amino acid, integrin-targeted bifunctional synthetic peptide (polylysine-molossin), and two (Lys)(16)-containing control peptides, were assessed for ex vivo gene delivery to the rabbit cornea. Critical physical properties of polylysine-molossin/DNA complexes were evaluated and both chloroquine and a 20 amino acid fusogenic peptide were used to promote endocytic exit., Results: Polylysine-molossin/DNA complexes and (Lys)(16)/DNA complexes at 10 microg/ml of DNA were much smaller and much more positively charged in non-ionic isotonic medium (5% dextrose or 5% dextrose buffered to pH 7.4 in 10 mM Tris) when compared with culture medium or phosphate-buffered saline (PBS). Addition of the fusogenic peptide (net charge -5) reversed the positive charge of complexes in PBS, and reduced the strong positive charge of polylysine-molossin/DNA complexes in dextrose. Polylysine-molossin/DNA complexes in 5% dextrose were much more effective for gene delivery to the cornea when compared with complexes in culture medium, and the fusogenic peptide was much more effective than chloroquine for promoting gene delivery. The optimal DNA/polylysine-molossin/fusogenic peptide w/w ratio was 1 : 3 : 2 at 10 microg/ml of DNA. Essentially 100% of corneal endothelial cells were transfected under these optimal conditions, without any evidence of toxicity. Integrin-targeting did not contribute significantly to gene delivery in this system., Conclusions: This DNA vector system, consisting entirely of synthetic peptides, is ideally suited for clinical applications of gene therapy of the corneal endothelium., (Copyright 2004 John Wiley & Sons, Ltd.)

Published

2004

42. The 50th anniversary of tolerance.

Author

Fabre JW

Subjects

Animals, History, 20th Century, Humans, Immunosuppression Therapy history, Transplantation Immunology

Published

2003

43. Modulation of adenovirus infection in vitro by antisense oligodeoxynucleotides.

Author

Whitehead BF, Schofield R, Rogers KM, Gustafsson K, and Fabre JW

Subjects

Adenoviridae genetics, Adenoviridae isolation & purification, Adenoviridae Infections genetics, Biological Assay, Cell Line, Humans, Lung virology, Oligodeoxyribonucleotides, Antisense therapeutic use, Adenoviridae drug effects, Adenoviridae Infections drug therapy, Cytopathogenic Effect, Viral drug effects, Oligodeoxyribonucleotides, Antisense pharmacology

Abstract

Objective: Antisense oligodeoxynucleotides (ODNs) may represent a novel, airway directed approach to the treatment of adenovirus infection of the lung, for which no specific therapy exists. This study assessed the efficacy of antisense ODNs in modulating adenovirus infection in vitro., Methodology: A biological assay, which quantified viral plaque formation by wild type adenovirus 5 in a lung epithelial cell line (A549), was used to evaluate the inhibitory effect of a number of antisense ODNs targeted to the early (E) 1 A and protein IX genes of adenovirus 5. Antisense ODNs (20-21mers, phosphorothioate end-protected) were designed to straddle the initiation of translation (AUG) codon of the mRNA of the targeted gene., Results: There was a consistent and significant (P < 0.005) reduction in viral plaque formation in those cells treated with an E1A antisense ODN, compared with the nonsense control ODN. Neither the addition of a cationic lipid (Lipofectamine), nor increasing the concentration of ODN from 1 micro mol to 15 micro mol enhanced the original inhibitory effect observed with the E1A antisense ODN., Conclusions: An antisense ODN targeted to the E1A gene can specifically inhibit adenovirus 5 infection in vitro, suggesting a potential therapeutic role for antisense ODNs in adenovirus infection of the lung.

Published

2003

44. Efficient gene delivery to primary neuron cultures using a synthetic peptide vector system.

Author

Collins L, Asuni AA, Anderton BH, and Fabre JW

Subjects

Animals, Antirheumatic Agents pharmacology, Cation Exchange Resins pharmacology, Cells, Cultured, Cerebral Cortex cytology, Chloroquine pharmacology, Dose-Response Relationship, Drug, Drug Interactions, Female, Fetus, Gene Expression, Gene Transfer Techniques, Genes, Reporter drug effects, Genes, Reporter physiology, Genetic Vectors genetics, Hemagglutinins, Indicators and Reagents pharmacology, Lipids pharmacology, Luciferases metabolism, Oligopeptides metabolism, Plasmids genetics, Pregnancy, Rats, Rats, Sprague-Dawley, Viral Proteins, beta-Galactosidase biosynthesis, Carrier Proteins genetics, Crotalid Venoms genetics, Glycoside Hydrolases, Hemagglutinins, Viral, Neurons physiology, Oligopeptides genetics, Peptide Fragments genetics, Transfection methods

Abstract

A bi-functional, 31 amino acid synthetic peptide (polylysine-molossin) was evaluated for gene delivery to primary cultures of rat cerebral cortex neurons. Polylysine-molossin consists of an amino terminal domain of 16 lysines for electrostatic binding of DNA, and a 15 amino acid, integrin-binding domain at the carboxyl terminal. High levels of gene delivery were obtained with 20-30 microM chloroquine, with a synthetic fusogenic peptide at an optimal DNA:polylysine-molossin:fusogenic peptide w/w ratio of 1:3:0.2, and with the addition of low concentrations of Lipofectamine 2000 at an optimal DNA:polylysine-molossin:Lipofectamine 2000 w/w ratio of 1:3:0.5. With the best combination, >30% of neurons strongly expressed the beta-galactosidase reporter gene, with no observable toxicity. DNA concentrations >2 microgram/ml were essential for efficient gene delivery. This synthetic peptide provides a safe, readily standardised and flexible DNA vector system well suited to ex vivo gene delivery to neurons for experimental and clinical applications.

Published

2003

45. The in vivo use of chloroquine to promote non-viral gene delivery to the liver via the portal vein and bile duct.

Author

Zhang X, Sawyer GJ, Dong X, Qiu Y, Collins L, and Fabre JW

Subjects

Administration, Oral, Animals, Antimalarials blood, Antimalarials pharmacokinetics, Bile Ducts metabolism, Chloroquine blood, Chloroquine pharmacokinetics, DNA therapeutic use, Gene Transfer Techniques, Injections, Intraperitoneal, Liver metabolism, Male, Portal Vein metabolism, Rats, Antimalarials pharmacology, Carrier Proteins administration & dosage, Carrier Proteins drug effects, Carrier Proteins therapeutic use, Chloroquine pharmacology, Crotalid Venoms administration & dosage, Crotalid Venoms therapeutic use, Genetic Vectors administration & dosage, Genetic Vectors drug effects, Genetic Vectors therapeutic use, Peptide Fragments administration & dosage, Peptide Fragments drug effects, Peptide Fragments therapeutic use

Abstract

Background: Assistance with exit from endocytic vesicles is a key factor for non-viral gene delivery, and is a particular challenge in vivo. We have evaluated the in vivo use of chloroquine administered systemically, orally and/or locally for gene delivery to the liver., Methods: The DNA vector (polylysine-molossin) is a 31 amino acid bifunctional synthetic peptide, incorporating an amino terminal chain of 16 lysines for electrostatic binding of DNA. Gene delivery was to the right lateral lobes of the liver by branches of the bile duct or portal vein., Results: Single intraperitoneal injections of 8, 25 and 75 mg/kg of chloroquine (the maximum tolerated single intraperitoneal dose) resulted in increasing levels of luciferase reporter gene expression, following gene delivery via the bile duct. 100 mg/kg of chloroquine orally was equivalent to 25 mg intraperitoneally. A 3-day course of intraperitoneal and oral chloroquine gave approximately 10-30-fold higher gene expression than an optimal single dose, and resulted in a scattering of positive hepatocytes in the lobule. Gene delivery via the bile duct was much more effective than via the portal vein. Serum chloroquine levels at the time of gene delivery showed a highly significant correlation with gene expression, but the maximum achievable levels in vivo ( approximately 1-2 micro M) were much lower than those required for optimal in vitro gene delivery. Chloroquine (0.2-5 mM) was also given locally in the bile duct with vector/DNA complexes. Maximum gene expression was obtained with 0.5 mM local chloroquine, but the level of gene expression was only equivalent to the 25 mg intraperitoneal dose., Conclusions: The in vivo use of chloroquine is effective for promoting gene delivery to the liver, but requires multiple dosing and is limited by systemic toxicity., (Copyright 2002 John Wiley & Sons, Ltd.)

Published

2003

46. The last unknown fact.

Author

Fabre JW

Subjects

Allergy and Immunology, Research, History of Medicine, Knowledge

Published

2002

47. In vivo gene delivery via portal vein and bile duct to individual lobes of the rat liver using a polylysine-based nonviral DNA vector in combination with chloroquine.

Author

Zhang X, Collins L, Sawyer GJ, Dong X, Qiu Y, and Fabre JW

Subjects

Animals, Bile Ducts, Binding Sites, Chloroquine administration & dosage, Crotalus, Dose-Response Relationship, Drug, Drug Administration Routes, Gene Expression, Genes, Reporter, Humans, Integrins metabolism, Liver, Male, Mice, Mice, Inbred BALB C, Portal Vein, Rats, Rats, Inbred Strains, Tumor Cells, Cultured, Chloroquine pharmacology, Crotalid Venoms, Gene Transfer Techniques, Genetic Vectors, Oligopeptides, Polylysine

Abstract

The objective of this study was to evaluate a bifunctional synthetic peptide as a DNA vector for regional gene delivery to the rat liver by the portal vein and bile duct routes. The 31-amino-acid peptide (polylysine-molossin) comprises an amino-terminal chain of 16 lysines for electrostatic binding of DNA, and the 15 amino acid integrin-binding domain of the venom of the American pit viper, Crotalus molossus molossus. Initial in vitro evaluation demonstrated that polylysine-molossin/DNA complexes were much smaller (approximately 50-100nm versus 500-1300nm), more positively charged, and more stable in isotonic dextrose in comparisons with salt-containing solutions. However, polylysine-molossin/DNA complexes in any solution other than complete culture medium were ineffective for gene delivery in vitro. Vector localization studies demonstrated that both the portal vein and bile duct routes provided excellent access of polylysine-molossin/DNA complexes to the liver. However, complexes delivered by the portal vein were rapidly lost (<15 min) following re-establishment of the portal circulation, whereas complexes delivered by the bile duct persisted much longer. Polylysine-molossin/DNA complexes in various isotonic solutions were delivered to the right lateral lobes either by perfusion through a branch of the portal vein or by infusion into appropriate branches of the bile duct. Two or three hours before gene delivery, rats were given a single injection of chloroquine. We report that the polylysine-molossin vector is much more effective (>10-fold) when delivered by the bile duct route with all isotonic solutions evaluated, and that polylysine-molossin/DNA complexes in isotonic dextrose are much more effective (>10-fold) than complexes in salt-containing solutions.

Published

2001

48. A powerful cooperative interaction between a fusogenic peptide and lipofectamine for the enhancement of receptor-targeted, non-viral gene delivery via integrin receptors.

Author

Zhang X, Collins L, and Fabre JW

Subjects

Amino Acid Motifs, Amino Acid Sequence, Binding, Competitive, Carrier Proteins chemistry, Cell Line, Crotalid Venoms chemistry, Genes, Reporter, Genetic Vectors, Hemagglutinins chemistry, Humans, Lipids, Molecular Sequence Data, Peptide Fragments chemistry, Tumor Cells, Cultured, Viral Proteins chemistry, Carrier Proteins metabolism, Cation Exchange Resins metabolism, Crotalid Venoms metabolism, Hemagglutinins metabolism, Hemagglutinins, Viral, Integrins metabolism, Lipid Metabolism, Peptide Fragments metabolism, Transfection methods, Viral Proteins metabolism

Abstract

Background: Following receptor-mediated endocytosis, vector/DNA complexes require assistance to exit endocytic vesicles in order to avoid degradation in the lysosomes. Overcoming this barrier is a major challenge for the development of receptor-targeted, non-viral gene delivery., Methods: The fusogenic peptide of influenza virus haemagglutinin, lipofectamine and chloroquine were tested singly and in combination in various doses for promoting in vitro gene transfer by an integrin-targeted, non-viral DNA vector (polylysine-molossin)., Results: The fusogenic peptide and lipofectamine both individually promoted integrin-targeted gene delivery. However, the combined use of these agents was particularly effective, even at concentrations where neither agent singly had any effect on promoting gene delivery by polylysine-molossin. This optimal combination was effective on several cell lines and primary cell cultures. On the HuH7 cell line, it was approximately five-fold more effective than optimal chloroquine concentrations for integrin-targeted gene delivery and four to five times more effective than commercially available polyethylenimine. With the beta-galactosidase reporter gene, 60-65% of HepG2 cells and 75-80% of HuH7 cells were positive. The surface charge of polylysine-molossin/DNA/lipofectamine/fusogenic peptide complexes was approximately the same as that of polylysine-molossin/DNA complexes. The size distribution of the complexes suggested that competitive binding of polylysine-molossin and lipofectamine to DNA influenced the overall efficacy of this approach., Conclusions: Although the mechanisms are not clear, the combined use of very low doses of two membrane-destabilizing agents results in high levels of receptor-targeted gene delivery.

Published

2001

49. The allogeneic response and tumor immunity.

Author

Fabre JW

Subjects

HLA Antigens immunology, Humans, Neoplasms physiopathology, Peptides immunology, T-Lymphocytes physiology, Transplantation, Homologous, Immunotherapy, Isoantigens immunology, Major Histocompatibility Complex immunology, Neoplasms immunology, T-Lymphocytes immunology

Abstract

The strong allogeneic response to donor MHC molecules in transplantation and the weak response to tumor antigens represent two important and divergent but potentially interactive immune responses. A patient's response to allogeneic MHC molecules might promote an effective T-cell response to self MHC-restricted tumor peptides and the possibilities for this are discussed here. These allogeneic responses might successfully be harnessed to promote the immune eradication of metastatic cancer.

Published

2001

50. Prospects for genetic manipulation of donor organs and tissues.

Author

Fabre JW

Subjects

Gene Expression, Humans, Tissue Donors, Transgenes genetics, Cornea metabolism, Corneal Transplantation physiology, Genetic Therapy trends

Published

2001