Your search keyword '"Davies AJ"' showing total 10 results

1. The effect of ricin B chain on the intracellular trafficking of an A chain immunotoxin.

Author

Timar J, McIntosh DP, Henry R, Cumber AJ, Parnell GD, and Davies AJ

Subjects

Antibodies, Monoclonal metabolism, Endocytosis, Gold Radioisotopes metabolism, Humans, Immunotoxins chemistry, Ricin chemistry, Tumor Cells, Cultured metabolism, Urinary Bladder Neoplasms metabolism, Cytoplasm metabolism, Immunotoxins metabolism, Ricin metabolism

Abstract

Covalent linkage of the A chain of ricin to the LICR-LOND-Fib75 monoclonal antibody produced an immunotoxin, Fib75-SS-ricin A, which demonstrated immunospecific toxicity to human bladder carcinoma cells in tissue culture (Forrester et al., 1984). The present studies have shown that ricin B chain potentiates the toxicity of the immunotoxin by two orders of magnitude and also significantly increases the rate of protein synthesis inhibition. Using immunoelectron microscopy, the receptor-mediated endocytosis and intracellular routing of the immunotoxin was studied with and without ricin B chain treatment after immunolocalisation of the conjugate. Fib75-SS-ricin A was internalised by the EJ cells predominantly in uncoated pits and vesicles and directed to the endosomes. Some degradation of the complex appeared to take place in multivesicular endosomes at early timepoints and 24 h after internalisation, most of the immunotoxin was found in lysosomes. Some ricin A chain epitopes were detected in Golgi vesicles. Cells treated with immunotoxin and ricin B chain endocytosed the complex predominantly in coated pits and coated vesicles. Using pre-embedding immunoperoxidase techniques, ricin chains were found in the whole Golgi complex and most of the conjugate escaped lysosomal degradation. Internalised immunotoxin was recycled back to the plasma membrane in an active form associated with vesicles which appeared to be derived predominantly from multivesicular endosomes. A similar mode of recycling has recently been reported (McIntosh et al., 1990) for ricin holotoxin in the same cell line. These observations may explain the potentiating effect of toxin B chains in the antibody-directed targeting of toxin A chains.

Published

1991

2. The vascularity of cutaneous melanoma: a quantitative histological study of lesions 0.85-1.25 mm in thickness.

Author

Carnochan P, Briggs JC, Westbury G, and Davies AJ

Subjects

Adult, Follow-Up Studies, Humans, Lymphocytes pathology, Melanoma pathology, Neoplasm Recurrence, Local, Prognosis, Recurrence, Regional Blood Flow, Skin blood supply, Skin Neoplasms pathology, Endothelium, Vascular pathology, Melanoma blood supply, Skin Neoplasms blood supply

Abstract

The vascularity of 107 primary cutaneous melanomas has been characterized by morphometric histological analysis. The lesions selected for study were of thickness 0.85-1.25 mm and the aim was to evaluate the prognostic significance of tumour vascularity. Two groups of patients were identified; 86 with no evidence of recurrence after a minimum follow-up period of 5 years and 21 with locoregional recurrence and/or metastasis. The lectin Ulex europaeus type I was used for endothelial cell staining of tissue sections and morphometric analysis was performed to derive the vascular length, surface and volume density from independent measurements of tumour, adjacent dermis and the junctional zone between tumour and underlying tissue. A wide range of values was obtained for each parameter with increased vascularity always found at the tumour base compared with the tumour as a whole. In relation to the adjacent normal dermis, vascularity was generally found to be higher at the tumour base but either higher or lower in the tumour overall. Tumour recurrence could not be predicted by any of the derived vascular parameters either independently or together with other histological and clinical features. This study suggests that tumour vascularity is of no prognostic significance in melanoma of the above thickness range. The highly variable extent of tumour vascularity was not correlated with other clinical or histological parameters, but may have implications for the delivery of pharmaceutical agents used for diagnosis or therapy.

Published

1991

3. Temporary inhibition of Moloney-murine sarcoma virus (M-MSV) induced-tumours by adoptive transfer of ricin-treated T-lymphocytes.

Author

Cerundolo V, Zanovello P, McIntosh D, Fabbris R, Davies AJ, and Collavo D

Subjects

Animals, Cell Survival drug effects, Epitopes immunology, Lymphocyte Culture Test, Mixed, Mice, Mice, Inbred C57BL, Moloney murine sarcoma virus immunology, Ricin therapeutic use, Sarcoma, Experimental immunology, Time Factors, Immunization, Passive, Ricin administration & dosage, Sarcoma, Experimental prevention & control, T-Lymphocytes, Cytotoxic immunology

Abstract

The potential use of tumour-specific T-lymphocytes loaded with ricin in cell targeting experiments was investigated. Moloney-murine sarcoma virus (M-MSV)-specific T-lymphocytes, obtained in mass mixed leucocyte-tumour cell culture (MLTC) and a M-MSV-specific cytotoxic T-lymphocyte (CTL) clone, were incubated with 125I-labelled ricin in order to evaluate toxin uptake and release. The internalized ricin (4.5 X 10(-17) mol and 6.5 X 10(-17) mol per 10(2) MLTC and CTL clone cells, respectively) was released rapidly during the first 30 min following treatment, and at a constant but slower rate over the next few hours. The cytotoxic activity of ricin-treated cells evaluated against antigen-related target cells, in a short term incubation 51Cr release assay, was unaffected during the first 30 min after treatment but decreased with time over the next few hours. However, the growth of antigen related as well as of unrelated tumour cells was strongly inhibited by the addition of ricin-treated cells to the culture system, thus indicating that released ricin is toxic for untreated target cells. The in vivo localization pattern of ricin-treated radiolabelled MLTC cells was found to be comparable with that of untreated cells 1 h after i.v. injection into syngeneic sublethally irradiated mice. After 6 h, however, more radiolabel was recovered from the liver of mice receiving ricin-treated MLTC cells. Ricin-treated M-MSV-specific T-lymphocytes were injected i.v. into tumour bearing sublethally irradiated mice. A temporary tumour growth inhibition (up to 6 days) was achieved following transfer of low doses of ricin-treated MLTC or CTL clone cells (1 X 10(6) and 0.5 X 10(6), respectively). In contrast, in M-MSV injected control mice, receiving only free toxin (from 5 to 20 ng) or untreated tumour-specific effector cell tumours grew progressively. The therapeutic effect was apparently specific since the injection of ricin-treated alloreactive T-lymphocytes did not influence tumour growth. These results suggest that M-MSV-specific T-lymphocytes loaded with ricin can deliver toxin to the target tumour mass and have a transient therapeutic effect.

Published

1987

4. Binding of peanut lectin to germinal-centre cells: a marker for B-cell subsets of follicular lymphoma?

Author

Rose ML, Habeshaw JA, Kennedy R, Sloane J, Wiltshaw E, and Davies AJ

Subjects

Adolescent, Adult, Aged, Arachis, Cells, Cultured, Child, Preschool, Fluorescein-5-isothiocyanate, Fluoresceins, Horseradish Peroxidase, Humans, Lymph Nodes immunology, Middle Aged, Palatine Tonsil immunology, Phenotype, Plant Lectins, Receptors, Immunologic analysis, Thiocyanates, B-Lymphocytes immunology, Lectins immunology, Lymphoma immunology

Abstract

The binding of horseradish-peroxidase-labelled peanut lectin (HRP-PNL) to cryostat sections of tonsil, lymphoma lymph nodes, reactive lymph nodes and miscellaneous tumours demonstrated that PNL binds selectively to lymphocytes in germinal centres. Lymph nodes from 21 patients with non-Hodgkin's lymphomas were phenotyped as cell suspensions for PNL binding, and the following surface markers: E rosetting, C3d, SIg, OK markers of T-cell subsets, Ig heavy-chain and light-chain classes. There was a positive correlation between PNL binding and cells with SIg and C3d receptors. 4/5 cases of centroblastic/centrocytic follicular lymphoma had a PNL+ SIg+ C3d+ phenotype. Both cases of centroblastic/centrocytic diffuse lymphoma were PNL-. There was no correlation between PNL binding and heavy- or light-chain Ig class. PNL binding and presence of C3d receptors were not always positively correlated, indicating that follicular cells may be either PNL+ SIg+ C3d+ or PNL+ SIg+ C3d-. The binding pattern of PNL to 1 case of thymic hyperplasia and 2 cases of malignant lymphoma lymphoblastic T type suggested that some but not all cortical thymocytes bind PNL.

Published

1981

5. The failure of human leukocyte interferon to influence the growth of human glioma cell populations: in vitro and in vivo studies.

Author

Bradley NJ, Darling JL, Oktar N, Bloom HJ, Thomas DG, and Davies AJ

Subjects

Adult, Aged, Animals, Antineoplastic Combined Chemotherapy Protocols therapeutic use, Carmustine administration & dosage, Cell Line, Female, Humans, Interferon Type I administration & dosage, Male, Mice, Mice, Inbred CBA, Middle Aged, Neoplasm Proteins biosynthesis, Neoplasm Transplantation, Procarbazine administration & dosage, Astrocytoma drug therapy, Brain Neoplasms drug therapy, Interferon Type I therapeutic use

Abstract

Five high-grade (3 grade III and 2 grade IV) astrocytoma tumour cell populations were treated with a preparation of Human Leukocyte Interferon either in monolayer cell culture or as multicellular spheroids in vitro or as xenografts growing in immune-deprived mice in vivo. A moderate and transient sensitivity was seen in one grade III tumour when tested in both of the in vitro assays, but no inhibition of growth was seen in vivo. Two tumours which were apparently resistant to Interferon treatment responded to orthodox chemotherapy. When used in conjunction with BCNU, Interferon was not effective in prolonging delay in tumour growth. It is concluded that Interferon is unlikely to be an effective agent in the treatment of malignant brain tumours.

Published

1983

6. Growth of human gliomas in immune-deficient mice: a possible model for pre-clinical therapy studies.

Author

Bradley NJ, Bloom HJ, Davies AJ, and Swift SM

Subjects

Animals, Astrocytoma pathology, Humans, Immunosuppression Therapy, Karyotyping, Medulloblastoma pathology, Mice, Mice, Inbred CBA, Mice, Nude, Neoplasm Transplantation, Neoplasms, Experimental pathology, Time Factors, Transplantation, Heterologous, Brain Neoplasms pathology, Disease Models, Animal, Glioma pathology

Abstract

Thirteen gliomas from 55 neurosurgical specimens, derived from 25 adults and 30 children, have been successfully grown as subcutaneous xenografts in immune-deprived or nude mice. Only 2 of the 30 paediatric specimens implanted (6.7%), a medulloblastoma and an astrocytoma Grade III, have grown compared with 11 of the 25 adult specimen (44%) which were mostly astrocytomas Grade III. Tumour growth usually occurred several months after implantation, and karyotypic analysis confirmed their human origin in all cases. The histopathology of xenografted tumours correlated with the original surgical material, both after initial implantation and when tumours had been passaged several times. Observations on tumour growth in various types of immune-deprived mice indicated that, within certain limits, the immunological competence of the host mouse did not relate to take rates of primary implants, but could affect the take rate of passaged tumours.

Published

1978

7. Effect of Pasteurella pneumotropica on the growth of transplanted Walker sarcoma cells.

Author

Simpson W, Simmons DJ, and Davies AJ

Subjects

Animals, Cell Line, Mice, Mice, Inbred CBA, Mice, Nude, Neoplasm Transplantation, Rats, Rats, Inbred Strains, Sarcoma, Experimental immunology, T-Lymphocytes immunology, Transplantation, Homologous, Pasteurella immunology, Sarcoma, Experimental prevention & control

Published

1980

8. Assessment of drug sensitivity of human leukaemic myeloblasts. I. Labelling human myeloblasts with 125IUdR for survival studies in mice.

Author

Falcão RP, Sonis S, MacLennan IC, Chassoux D, Davies AJ, and Munro TR

Subjects

Animals, Blood Cells metabolism, Bone Marrow Cells, Cell Survival drug effects, Cells, Cultured, Freezing, Idoxuridine metabolism, In Vitro Techniques, Isotope Labeling methods, Leukemia, Myeloid, Acute metabolism, Mice, Drug Evaluation, Preclinical methods, Leukemia, Myeloid, Acute drug therapy

Abstract

The compound (125)IUdR can be incorporated in a stable form into the DNA of cells. The isotope is released if labelled cells or their progeny die. Consequently the rate of (125)I excretion from mice can be used to follow the fate of labelled cells in vivo. Using these principles we show:(1) Sufficient label can be incorporated in vitro into both fresh and cryopreserved human leukaemic myeloblasts, in non-toxic concentrations, to allow their survival in mice to be estimated by whole-body counting;(2) The release of isotope from labelled cells is sufficiently slow to offer reasonable expectation that this technique can be used for assessing the sensitivity of myeloblasts to cytotoxic agents in vivo (an application described in the second paper in this series, Sonis, Falcão and MacLennon, 1977);(3) The rate of (125)Iexcretion from mice injected with myeloblasts from different donors varies. This probably reflects different rates of spontaneous death of injected myeloblasts;(4) Active rejection of myeloblasts starts within 48 h of their injection into mice;(5) Indirect evidence that phagocytic cells may be active agents in myeloblast destruction in mice;(6) Various methods of immunologically depriving mice were assessed to see if they would result in a useful increase in survival of injected human myeloblasts. We conclude that there is little advantage and some limitations in using mice thus deprived;(7) One of the agents used for immunological deprivation-silica powder-markedly decreased the rate of (125)I loss from mice injected with labelled killed myeloblasts. This experience emphasizes the importance of including the killed-cell control in this assay.

Published

1977

9. Anaemia associated with the NK/lymphoma in mice.

Author

DAVIES AJ, CROSS AM, and LAPIS K

Subjects

Animals, Mice, Anemia, Lymphoma, Neoplasms, Neoplasms, Experimental

Published

1962

10. Attempted Tumour Therapy Complicated by a Viroid Associate of the Tumour.

Author

Lapis K and Davies AJ

Published

1962