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9. A suppressor of a wtf poison-antidote meiotic driver acts via mimicry of the driver’s antidote.

Author

Bravo Núñez, María Angélica, Lange, Jeffrey J., and Sarah, Zanders E.

Subjects
MEIOTIC drive, GAMETOGENESIS, ANTIDOTES, GENOMES, SCHIZOSACCHAROMYCES
Abstract

Meiotic drivers are selfish alleles that subvert gametogenesis to increase their transmission into progeny. Drivers impose a fitness cost, putting pressure on the genome to evolve suppressors. Here we investigate the wtf gene family from Schizosaccharomyces pombe, previously shown to contain meiotic drivers in wild isolates. We discovered that wtf13 found in lab stocks is a meiotic driver. wtf13 kills spores that do not inherit it by generating both a diffusible poison and a spore-specific antidote. Additionally, we demonstrate that wtf13 is suppressed by another wtf gene, wtf18-2, that arose spontaneously in the lab and makes only an antidote. Wtf18-2 does not act indiscriminately to prevent spore destruction. Instead, it rescues only the spores that inherit wtf18-2. In this way, wtf18-2 selfishly gains a transmission advantage of its own while dampening the drive of wtf13. This establishes a novel paradigm for meiotic drive suppressors and provides insight into the mechanisms and evolution of drive systems. [ABSTRACT FROM AUTHOR]

Published
2018
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13. Secondary immunoglobulin responses of BALB/c mice previously stimulated with goat anti-mouse IgD

Author

Champion, B R, Buckham, S, Page, K, Obray, H, and Zanders, E D

Subjects
Mice, Mice, Inbred BALB C, Interleukin-6, Goats, Immunoglobulin G, Animals, Female, Immunoglobulin D, Immunoglobulin E, Immunologic Memory, Research Article, Antibodies, Anti-Idiotypic, Immunoglobulin A
Abstract

Intravenous injection of goat antibodies to mouse IgD (GAMD) into BALB/c mice has been shown to induce vigorous T-cell dependent immunoglobulin responses, particularly of the IgG1 and IgE isotypes. We have confirmed these findings and show that IgA responses are also triggered in this model. Since the study of IgE regulation in allergic individuals is concerned with secondary and subsequent T- and B-cell responses, we boosted GAMD-primed mice with goat antibodies to IgE or IgA in an attempt to specifically retrigger IgE- and IgA-bearing memory B cells. However, we found that secondary IgG1, IgE and IgA production could be elicited equally well by either antibody preparation or by normal goat IgG (GIg). As with the primary response, GIg primed and boosted mice produced very low or undetectable IgG1, IgE and IgA responses. These data suggest that GAMD is very efficient at priming T cells specific for GIg epitopes and that once primed they can be readily re-triggered by GIg. Spleen cells taken 7 days after boosting GAMD-primed mice were found to spontaneously produce much higher levels of interleukin-6 (IL-6) in culture than cells from unboosted or GIg primed and boosted mice. In contrast to primary responses, where IgE levels return to background (less than 40 ng/ml) very quickly, circulating IgE levels in boosted mice initially declined before reaching a plateau level (approximately 1 microgram/ml) which was maintained for at least 148 days. IgG1 and IgA levels continued to fall over this same time period. Mice which had been primed (but not boosted) 10 months earlier were all found to have detectable IgE in their blood, despite the fact that following priming IgE becomes undetectable within 2-3 weeks. Since only a part of the IgE response was directed towards the antigen (GIg), these observations suggest the possibility that B cells initially primed to make IgE can be non-specifically retriggered in vivo.

Published
1991

14. The dissociation of interleukin-2 production and antigen-specific helper activity by clonal analysis.

Author

Lamb, J. R., Zanders, E. D., Feldmann, M., Lake, P., Eckels, D., Woody, J. N., and Beverley, P. C. L.

Subjects
*INTERLEUKINS, *ANTIGENS, *INFLUENZA viruses, *T cells, *PHENOTYPES, *IMMUNOGLOBULINS
Abstract

Influenza virus immune human T-lymphocyte clones maintained in continuous culture in TCGF were analysed for helper activity and interleukin-2 (IL-2) production. The clones that functioned as helper cells in the production of specific antibody failed to release detectable amounts of IL-2. Conversely, the T cells that produced IL-2 were unable to provide either specific or non-specific helper function. These findings indicated the IL-2 is not an essential component for helper activity. However, phenotypic analysis revealed that both the functional subsets of T-cell clones expressed the helper phenotype in that they were T4+, T3+ and T11+ Nevertheless analysis with other antibodies revealed differences in that the IL-2 releasing clone showed greater staining with the anti-T-cell subset antibodies 9.3 and Leu 8, confirming that there is phenotype as well as functional heterogeneity within the helper inducer T-cell population. [ABSTRACT FROM AUTHOR]

Published
1983

15. Antigen-specific and non-specific helper activities derived from supernatants of human influenza virus-specific T-cell lines.

Author

Zanders, E. D., Fischer, A., Smith, Susan, Beverley, P. C. L., and Feldmann, M.

Subjects
*CELL culture, *INFLUENZA viruses, *T cells, *CELL lines, *IMMUNOGLOBULINS, *INTERLEUKINS
Abstract

A T-cell line (H3) was established by culturing human peripheral blood mononuclear cells with influenza virus A/X31 and maintained in long term culture with Interleukin-2 (TCGF). Supernatants were prepared by culturing these cells overnight in the absence of Interleukin-2 but with A/X31 and irradiated autologous E rosette negative cells as a source of antigen presenting cells, and harvesting by centrifugation. The supernatants were shown to replace T cells in helping E- (B) cells to produce antibody specific to A/X31 which was measured by enzyme immunoassay (EIA). Although maximal help was obtained with autologous or semi allogeneic B cells (in the latter case bearing HLA-DR 3 loci) there was still significant antibody production with allogeneic combinations. The supernatants were subsequently fractionated into specific and non-specific helper activities by gel filtration, giving an approximate tool. wt of 50–70,000 and 10–30,000 for each respectively. The specific HF was shown to be genetically restricted in its action upon B cells and also to generate antibody to A/X31 only. The lower molecular weight material acted on any responding B cell regardless of H LA-DR type and produced antibody non-specifically in culture with E- cells even in the absence of antigen. The apparent lack of restriction was therefore due to the masking effect of non-specific and non-restricted HF(s) on the genetically restricted specific HF produced by this line. [ABSTRACT FROM AUTHOR]

Published
1983

16. Partial characterization of murine and monkey helper factor to a streptococcal antigen.

Author

Zanders, E. D., Lamb, J. R., Kontiainen, Sirkka, and Lehner, T.

Subjects
*IMMUNE response, *ANTIGENS, *STREPTOCOCCUS, *GLYCOPROTEINS, *ENZYMES, *CELLS
Abstract

Helper factors specifically stimulating cooperative antibody responses by normal mouse spleen cells to a dinitrophenylated protein antigen from Streptococcus mutans (DNP-SA) were produced in vitro from monkey peripheral blood leucocytes and mouse spleen cells. The factors were partially characterized by gel filtration on Sephadex G-75, isoelectric focusing, treatment with heat and degradative enzymes and binding to specific immunoadsorbents. Gel filtration of both the monkey and mouse factors showed coelution with human serum albumin, suggesting a molecular weight of approximately 70,000. The isoelectric points fell within the range of 4·9-5·2 for monkey and 6·4-6·7 for the mouse helper factors. The glycoprotein nature of both factors was suggested by their lability to heat and sensitivity to pronase and neuraminidase. The factors carried a small fragment of the stimulating antigen and showed specific binding to SA but not to keyhole limpet haemocyanin (KLH). Monkey factor bound to rabbit antisera directed against the Fc portion of monkey IgM, but not to the IgG or IgA isotypes. The mouse factor contained determinants coded for by the I-Ak but not I-Jk subregion of the MHC. Both factors were absorbed by an antisenim to helper factor raised in rabbits against a KLH-specific mouse helper factor as immunogen. A corresponding antisenim to suppressor factor failed to adsorb either factor. This emphasizes the specific identities of helper and suppressor factors and suggests an evolutionary relationship between those derived from monkey and mouse leucocytes. [ABSTRACT FROM AUTHOR]

Published
1980

17. Immunoregulation in the common marmoset, <em>Calithrix jaccus</em>: functional properties of T and B lymphocytes and their response to human interleukins 2 and 4.

Author

Quint, D. J., Buckham, S. P., Bolton, E. J., Solari, R., Champion, B. R., and Zanders, E. D.

Subjects
PRIMATES, IMMUNE response, IMMUNOLOGY, ANTIGEN-antibody reactions, T cells, B cells
Abstract

Non-human primates have been used to study immune function to a much lesser extent than readily available strains of inbred rodents. Nevertheless, in situations where it might be desirable, but impossible, to study human immune responses in vivo, lower primates could provide an acceptable alternative. In order to extend the knowledge of T- and B-lymphocyte function in lower primates, the common marmoset Callithrix jaccus was used as an experimental model. The functional similarities between this species and humans at the level of T-B co-operation in the antibody response were examined, and xenoreactive T-lymphocyte clones were obtained from marmoset spleen cells using Epstein—Barr virus (EBV)-transformed human B cells as stimulators. These clones could act as helper cells when co-cultured with human B lymphocytes, inducing the secretion of both IgM and IgG. Lymphokine production by mitogen-stimulated marmoset T-cell clones was also examined. Interleukins (IL) 2 and 4 activities were detected in clone supernatants using bioassays and interferon-gamma (IFN-γ) was detected using a solid-phase ELISA system. However, SDS—PAGE analysis of biosynthetically labelled marmoset and human T-cell clone supernatant proteins revealed major differences between the soluble T-cell products of the two species. The proliferative responses of marmoset T and B cells to recombinant human IL-2 and IL-4 were also examined. Stimulation of [3H]thymidine uptake was detected in both T cell- and anti-IgM-stimulated B-cell cultures with both of the lymphokines. These results suggests that the key components of the antibody response are functionally conserved between lower primates and man and that the common marmoset may be useful as an in vivo model of immune function, particularly with regard to the role of interleukins such as IL-2 and IL-4. [ABSTRACT FROM AUTHOR]

Published
1990

18. Functional and phenotypic analysis of human T-cells clones which stimulate IgE production <em>in vitro</em>.

Author

Quint, D. J., Bolton, E. J., McNamee, L. A., Solari, R., Hissey, P. H., Champion, B. R., Mackenzie, A. R., and Zanders, E. D.

Subjects
T cells, IMMUNOGLOBULIN E, IMMUNOGLOBULINS, B cells, INTERLEUKINS, INTERFERONS
Abstract

Peripheral blood mononuclear cells (PBMC) from a patient suffering from the hyper IgE syndrome were used to generate phytohaemagglutinin (PHA)-expanded T-cell clones (all CD4+, CD8-, CD23-). A selection of the clones was tested for their ability to help IgE secretion by culturing with normal B cells in the presence of solid-phase antibody to CD3. Supernatants were harvested on Day 7 and assayed by ELISA for IgE, IgG and IgM. Lymphokine secretion by the clones was assessed by culturing clones for 24 hr with solid-phase antibody to CD3 followed by assay of the supernatants for IL-2, IL-4 and interferon-gamma (IFN-γ) production. In addition, clones were analysed by flow cytometry for CDw29 and CD45R expression. Initial experiments with seven clones indicated that those clones that could help IgE secretion also stimulated optimal IgG and IgM responses. All clones appeared to secrete IL-2, IL-4 and IFN-γ, although the mounts of each varied. These results confirm recent findings that human T-cell clones do not fall into Tinf (Th1) and Th (Th2) type subsets as described in the muse. There was no clear correlation between the lymphokines secreted by the clones and their capacity to help IgE production. However, the helper function of the clones for all isotypes, including IgE, appeared to be related to the level of expression of the surface antigen CDw29. [ABSTRACT FROM AUTHOR]

Published
1989

19. An in vitro model of allergen-dependent IgE synthesis by human B lymphocytes: comparison of the response of an atopic and a non-atopic individual to Dermatophagoides spp. (house dust mite).

Author

O'Hehir, R. E., Bal, V., Quint, D., Moqbel, R., Kay, A. B., Zanders, E. D., and Lamb, J. R.

Subjects
IMMUNOGLOBULIN E, ALLERGENS, LYMPHOCYTES, DERMATOPHAGOIDES, B cells, INTERLEUKIN-4
Abstract

An allergen-dependent in vitro model of immunoglobulin E (IgE) synthesis by human B cells is reported. Using this model, it is demonstrated that polyclonal T cells and CD4+ Dermatophagoides spp. (house dust mite)-specific 1-cell clones derived from an atopic, house dust mite (HDM)-allergic individual are able to support IgE synthesis by autologous B cells. The helper activity was interleukin- 4 (IL-4) dependent as only cloned T cells expressing detectable mRNA for IL-'I were able to induce IgE synthesis without the addition of exogenous IL-4. Peripheral and cloned I cells reactive with HDM could also be identified from a non-atopic individual but neither population was able to support IgE production even in the presence of exogenous IL-4. [ABSTRACT FROM AUTHOR]

Published
1989

20. Functional evidence for a monoclonal antibody that binds to the human IL-4 receptor.

Author

Larche, M., Lamb, J. R., O'Hehir, R. E., Imami-Shita, N., Zanders, E. D., Quint, D. E., Moqbel, R., and Ritter, M. A.

Subjects
MONOCLONAL antibodies, INTERLEUKIN-4, T cells, CELL receptors, LYMPHOKINES, B cells
Abstract

The complex pleiotropic effects of the T-cell derived lymphokine interleukin-4 (IL-4) are becoming increasingly well documented; however, functional studies have been hampered by the lack of reagents directed against the receptor for this factor. In this report, we present data which suggest that the monoclonal antibody MR6 binds to the human interleukin-4 receptor (IL-4R). Addition of MR6 to cultures of T cells proliferating in response to IL-4 inhibited this response in a dose-dependent fashion, giving total inhibition at 10 μg/ml. Similarly, the IL-4-dependent production of specific antigen-induced IgE by B-cell populations was completely abrogated by MR6. Flow cytometric studies of the modulation of cell surface molecules after T-cell activation suggest that expression of the molecule detected by MR6 (p145-MR6) correlates inversely with that of the interleukin-2 receptor (IL-2R). These data, together with the previously determined molecular weight and tissue distribution of this molecule, strongly indicate that MR6 binds to the human IL-4R.. [ABSTRACT FROM AUTHOR]

Published
1988

21. Inositol lipid metabolism in human T lymphocytes activated via the T3 complex.

Author

Cockcroft, S., Lamb, J. R., and Zanders, E. D.

Subjects
LIPID metabolism, INOSITOL, LYMPHOCYTES, ANTIGENS, PHOSPHOINOSITIDES, IMMUNOGLOBULINS
Abstract

Cloned human T lymphocytes and a mitogenic monoclonal antibody (UCHT1) that binds to the T3 antigen complex were used to study the role of inositol lipid hydrolysis in T-cell activation. Binding of the T3 molecular complex with anti-T3 antibody induced the generation of inositol trisphosphate after a lag of 1 min. While this is commensurate with the rise in cytosolic Ca2+ in these cells, examination of the inositol lipid revealed that phosphorylation of phosphatidylinositol 4-phosphate to phosphatidylinositol 4,5-bisphosphate occurred before the generation of inositol trisphosphate. Thus, activation of an inositol lipid kinase appears to be one of the primary signals in cellular activation in human T lymphocytes. [ABSTRACT FROM AUTHOR]

Published
1987

24. Use of two-dimensional gel electrophoresis to measure changes in synovial fluid proteins from patients with rheumatoid arthritis treated with antibody to CD4.

Author

Smith, M A, Bains, S K, Betts, J C, Choy, E H, and Zanders, E D

Abstract

Synovial fluid proteins from microliter volumes of synovial fluid were resolved by two-dimensional polyacrylamide gel electrophoresis and detected by silver staining to investigate the feasibility of using two-dimensional (2D) electrophoresis in the clinical research setting and provide global disease information of disease progression. Several hundred proteins could be resolved as spots, many of which displayed the characteristic pattern of plasma-derived glycoproteins. The lowest level of detection was approximately 0.2 ng from a total of 50 microg of protein loaded. Most of the proteins could be identified on the basis of pI and molecular weight when compared with plasma protein maps on the World Wide Web. Unknown proteins were characterized by mass spectrometry of tryptic digests and by comparison with peptide databases. Synovial fluids from patients with rheumatoid arthritis were analyzed using this technique. Each subject received a fixed dose of antibody to CD4 as part of a phase II clinical trial to determine the efficacy of this immunosuppressive treatment in modifying disease activity. Synovial fluid was removed at day 0, followed by administration of antibody. Subsequent removal of synovial fluid and additional administration of antibody were carried out at different times thereafter. Changes in levels of acute-phase proteins were quantified by densitometry of silver-stained 2D polyacrylamide gels. Other parameters of disease progression such as serum C-reactive protein and physician's global assessment of clinical condition were used for comparison. In this way, changes in acute-phase proteins towards normal levels, as measured by 2D polyacrylamide gel electrophoresis, could be correlated with clinical improvement and conventional clinical chemistry measurements. Thus, the system can be used for quantitative analysis of protein expression in sites of autoimmune disease activity such as the synovial fluid of rheumatoid arthritis patients.

Published
2001
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25. Reverse transcriptase-PCR analysis of bacterial rRNA for detection and characterization of bacterial species in arthritis synovial tissue.

Author

Kempsell, K E, Cox, C J, Hurle, M, Wong, A, Wilkie, S, Zanders, E D, Gaston, J S, and Crowe, J S

Abstract

Onset of rheumatoid arthritis (RA) is widely believed to be preceded by exposure to some environmental trigger such as bacterial infectious agents. The influence of bacteria on RA disease onset or pathology has to date been controversial, due to inconsistencies between groups in the report of bacterial species isolated from RA disease tissue. Using a modified technique of reverse transcriptase-PCR amplification, we have detected bacterial rRNA in the synovial tissue of late-stage RA and non-RA arthritis controls. This may be suggestive of the presence of live bacteria. Sequencing of cloned complementary rDNA (crDNA) products revealed a number of bacterial sequences in joint tissue from each patient, and from these analyses a comprehensive profile of the organisms present was compiled. This revealed a number of different organisms in each patient, some of which are common to both RA and non-RA controls and are probably opportunistic colonizers of previously diseased tissue and others which are unique species. These latter organisms may be candidates for a specific role in disease pathology and require further investigation to exclude them as causative agents in the complex bacterial millieu. In addition, many of the detected bacterial species have not been identified previously from synovial tissue or fluid from arthritis patients. These may not be easily cultivable, since they were not revealed in previous studies using conventional in vitro bacterial culture methods. In situ hybridization analyses have revealed the joint-associated bacterial rRNA to be both intra- and extracellular. The role of viable bacteria or their nucleic acids as triggers in disease onset or pathology in either RA or non-RA arthritis controls is unclear and requires further investigation.

Published
2000

26. Immunochemical properties of antigen-specific monkey T-cell suppressor factor induced with a Streptococcus mutans antigen

Author

Lamb, J R, Zanders, E D, Kontiainen, S, and Lehner, T

Abstract

Antigen-specific suppressor factor could be released from monkey suppressor T cells induced in vitro with a protein antigen isolated from the carcinogenic bacterium Streptococcus mutans. The suppressor activity was due to the factor itself and not to carryover of free antigen. Characterization of the monkey factor revealed it to have a molecular weight of ca. 70,000, and to contain a constant region and determinants encoded by the major histocompatibility complex. The presence of immunoglobulin determinants could not be demonstrated. However, by virtue of its adsorption to specific antigen, an antigen-combining site was shown to be present. The possible regulatory role of streptococcal antigen-specific suppressor factor in protection against dental caries is discussed.

Published
1980
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27. Purification and characterization of recombinant human interleukin 4. Biological activities, receptor binding and the generation of monoclonal antibodies

Author

Solari, R, Quint, D, Obray, H, McNamee, A, Bolton, E, Hissey, P, Champion, B, Zanders, E, Chaplin, A, Coomber, B, Watson, M, Roberts, B, and Weir, M

Abstract

A synthetic gene coding for human interleukin 4 (IL-4) was cloned and expressed in Saccharomyces cerevisiae (baker's yeast) as a C-terminal fusion protein with the yeast prepro alpha-mating factor sequence, resulting in secretion of mature IL-4 into the culture medium (0.6-0.8 micrograms/ml). A protocol was developed for purification of this protein. Crude cell-free conditioned medium was passed over a concanavalin A-Sepharose affinity column; bound proteins were eluted and further purified by S-Sepharose Fast Flow cation exchange and C18 reverse-phase h.p.l.c. Highly purified IL-4 was obtained by this method (0.3-0.4 mg per litre of culture) with a recovery of 51%. Thermospray liquid chromatography-mass spectrometry showed the C-terminal N-glycosylation site to be largely unmodified, and also showed that the N-terminus of the purified recombinant IL-4 (rIL-4) was authentic. Thiol titration revealed no free cysteine residues, implying that there are three disulphide groups, the positions of which remain to be determined. We have characterized the biological activities of the purified rIL-4. This material is active in B-cell co-stimulator assays, T-cell proliferation assays and in the induction of cell-surface expression of CD23 (the low-affinity receptor for IgE) on tonsillar B-cells. Half-maximal biological activity of the rIL-4 was achieved at a concentration of 120 pM. We have radioiodinated rIL-4 without loss of biological activity and performed equilibrium binding studies on Raji cells, a human B-cell line. The 125I-rIL-4 bound specifically to a single class of binding studies on Raji cells, a human B-cell line. The 125I-rIL-4 bound specifically to a single class of binding site with high affinity (Kd = 100 pM) and revealed 1100 receptors per cell. Receptor-ligand cross-linking studies demonstrated a single cell-surface receptor with an apparent molecular mass of 124 kDa. Two monoclonal antibodies have been raised to the human rIL-4, one of which blocks both the biological activity of rIL-4 and binding to its receptor.

Published
1989
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28. Affinity purification and characterization of protease-susceptible antigen I of Streptococcus mutans

Author

Russell, M W, Zanders, E D, Bergmeier, L A, and Lehner, T

Abstract

An antigenic component (antigen I) of the cell surface of Streptococcus mutans has been purified from culture supernatants and shown to be immunologically identical to the protease-susceptible moiety of antigen I/II. Ion-exchange and gel filtration chromatography failed to yield a physicochemically homogeneous product. Immunoasbsorbent chromatography on single and tandem columns containing immobilized antibodies to antigens I/II and II yielded identical products which were homogeneous in sodium dodecyl sulfate-polyacrylamide gel electrophoresis, and which when injected into rabbits induced monospecific antisera to antigen I. This antigen consisted of approximately 70% protein. Its molecular weight was estimated as 150,000, and the isoelectric point was estimated to be 5.1. Immunofluorescence microscopy using monospecific antiserum to antigen I showed that a similar antigen was present on cells of S. mutans serotypes a, c, d, e, f, and g, but not b.

Published
1980
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29. Protein antigens of Streptococcus mutans: purification and properties of a double antigen and its protease-resistant component

Author

Russell, M W, Bergmeier, L A, Zanders, E D, and Lehner, T

Abstract

A surface protein antigen of Streptococcus mutans having two sets of antigenic determinants (antigens I and II) was purified by column chromatography from culture supernatants of S. mutans serotype c. The protease-resistant component, antigen II, was purified from pronase-digested antigen I/II. The antigens were analyzed chemically and immunologically, and their physicochemical properties were investigated. Antigen I/II consisted of more than 80% protein, and its peptide chain molecular weight was estimated to be 185,000. Antigen II consisted of approximately 60% protein, with a peptide chain molecular weight of 48,000. Antisera to antigens I/II and II were raised in rabbits and used to investigate the presence of the antigens in cells of other streptococci. This indicated that not only serotype c but also serotypes e and f possessed antigen I and II determinants, whereas serotypes a, d, and g possessed a determinant related to antigen I but not one related to antigen II.

Published
1980
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30. Inositol lipid metabolism in human T lymphocytes activated via the T3 complex

Author

Shamshad Cockcroft, Lamb, J. R., and Zanders, E. D.

Subjects
Time Factors, CD3 Complex, Inositol Phosphates, T-Lymphocytes, Antigens, Surface, Humans, Lymphocyte Activation, Phosphatidylinositols, Research Article
Abstract

Cloned human T lymphocytes and a mitogenic monoclonal antibody (UCHT1) that binds to the T3 antigen complex were used to study the role of inositol lipid hydrolysis in T-cell activation. Binding of the T3 molecular complex with anti-T3 antibody induced the generation of inositol trisphosphate after a lag of 1 min. While this is commensurate with the rise in cytosolic Ca2+ in these cells, examination of the inositol lipid revealed that phosphorylation of phosphatidylinositol 4-phosphate to phosphatidylinositol 4,5-bisphosphate occurred before the generation of inositol trisphosphate. Thus, activation of an inositol lipid kinase appears to be one of the primary signals in cellular activation in human T lymphocytes.

Published
1987

31. Genetically restricted and unrestricted antigen specific helper factors

Author

Feldmann, M, Fischer, A, Zanders, E, and Beverley, P

Abstract

Some human antigen specific helper factors (HF) derived from long term human T helper cell lines are genetically restricted in their action. Other human HF's, derived from 4-6 day cultures, are capable of activating mouse spleen cell cultures, and hence are not xenogeneically restricted. While it is possible that these results suggest a heterogeneity of HF, we have also found that some long term lines make both antigen specific HF and non specific factors. In this case the whole supernatant appears unrestricted but specific, suggesting a possible explanation for the variable degree of genetic restriction.

Published
1982

32. Nitrifikation, Denitrifikation und Blähschlammverhinderung bei Kläranlagen durch schubweise Abwasserzugabe

Author

Zanders, E.

Abstract

In der vorliegenden Arbeit wurde die Möglichkeit der Nitrifikation und Denitrifikation sowie der Blähschlammbekämpfung in Belebungsanlagen untersucht. Dazu wurden verschiedene Laborkläranlagen und halbtechnische Versuchsanlagen konstruiert, die mit diskontinuierlicher Abwasserzugabe betrieben werden konnten. Erste Versuche zur aeroben Nachreinigung von fermentiertem Brüdenkondensat zeigten, daß dieses gut abbaubar war, bei der Reinigung in Kläranlagen jedoch Blähschlamm verursachte. Mit einer Zugabe von Spurenelementen und Nährstoffen konnte die Entwicklung fadenförmiger Bakterien eingedämmt jedoch nicht verhindert werden. Bei diskontinuierlicher Beschickung der Laborkläranlagen mit fermentiertem Brüdenkondensat entwickelten sich vorrangig flockenbildende Bakterien und Blähschlamm konnte verhindert werden. Das in den Laborkläranlagen blähschlammverursachende fadenförmige Bakterium konnte isoliert, als Bacillus sp. erkannt und durch physiologische Tests näher beschrieben werden. Bei Versuchen mit halbtechnischen Kläranlagen wurde festgestellt, daß die diskontinuierliche Abwasserzugabe, bei unterschiedlichen Abwässern, eine für die Abwasserreinigung vorteilhafte Biezönese mit vorrangig flockenbildenden Bakterien begünstigt und den Reinigunsprozeß stabilisiert. Durch eine gesteuerte Belüftung, zusätzlich zur diskontinuierlichen Abwasserzugabe, konnte im Belebungsbecken eine vollständige Nitrifikation und Denitrifikation erreicht werden. Bei unterschiedlichen C:N-Verhältnissen im Zulauf von Laborkläranlagen wurden die jeweiligen Stoffumsatzraten der Nitrifikanten und Denitrifikanten bestimmt. Zum Nachweis der Denitrifikation wurde eine Stickstoffbilanz unter Berücksichtigung der partikulären, gelösten und gasförmigen Stickstoffverbindungen erstellt. Es wurde festgestellt, daß die möglichen Zwischenprodukte der Nitrifikation und Denitrifikation (N$_{2}$O, NO und NO$_{2}$ ) bei der diskontinuierlichen Abwasserzugabe mit gesteuerter Belüftung nur in geringen Spuren freigesetzt werden. Auf Grund der ermittelten Daten wurde, in Zusammenarbeit mit Ingenieuren, der Umbau einer Kläranlage mit 30.000 angeschlossenen Einwohnergleichwerten zur sukzedanen Nitrifikation/Denitrifikation geplant. Die umgebaute Kläranlage wird 1990 in Betrieb gehen.

Published
1989

39. Making sense of molecular signatures in the immune system.

Author

Davies NJ, Tadesse MG, Vannucci M, Kikuchi H, Trevino V, Sarti D, Dragoni I, Contestabile A, Zanders E, and Falciani F

Subjects
Animals, Autoimmune Diseases immunology, Gene Expression Profiling, Humans, Immune System immunology, Immune System ultrastructure, Inflammation immunology, Leukemia immunology, Lymphocytes immunology, Lymphocytes metabolism, Principal Component Analysis, Protein Array Analysis, Stem Cells immunology, Stem Cells metabolism, Stromal Cells immunology, Stromal Cells metabolism, Computational Biology, Genomics, Immune System chemistry
Abstract

The development of Functional Genomics technologies has opened new avenues to investigate the complexity of the immune system. Microarray technology has been particularly successful because of its relatively low cost and high genome coverage. Consequently to our ability to monitor the expression of a significant proportion of an organism genome, our understanding of the molecular dynamics behind cell differentiation and cell response has greatly improved. Molecular signatures associated to immune cells have provided important tools to investigate the molecular basis of diseases and have been often associated to diagnostic and prognostic markers. The availability of such large collection of data has stimulated the application of complex machine learning techniques in the attempt to link molecular signatures and cell physiology. Here we review the most recent developments in the analysis of molecular signatures in the immune system.

Published
2004
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40. [Influence of visual cues on upright postural control: differentiated effects of eyelids closure].

Author

Rougier P, Zanders E, and Borlet E

Subjects
Adult, Algorithms, Biomechanical Phenomena, Female, Gravitation, Humans, Male, Middle Aged, Movement physiology, Postural Balance physiology, Pressure, Cues, Eyelids physiology, Posture physiology, Vision, Ocular physiology
Abstract

In most protocols aimed at testing balance abilities, patients are generally required to close their eyes in order to gain insight about proprioceptive cues and the way the central nervous system (CNS) uses this information. However, one should not exclude possible interaction with the physiological mechanisms involved in eyelid closure, thus leading to a biased neurological evaluation. To assess this possible involvement, 15 healthy adults were required to keep their eyes open in the dark (YOn), to close normally (YF) and forcibly their eyelids (YFF), respectively in random order. The analysis was focused on elementary motions computed from the complex center of pressure (CP) trajectories, i.e. the horizontal motions of the center of gravity (CG(h)) and the difference between the CP and the vertical projection of the center of gravity (CP-CG(v)). The former is recognized as the main variable in postural control whilst several interesting features can be extracted from the latter: their link with the horizontal accelerations communicated to the CG, the level of muscular activity and the implied ankle stiffness expressed by their frequential distribution. The results indicate that the amplitudes of the CP-CG(v) spectra are statistically reduced in YOn when compared to the YF condition, especially in the antero-posterior direction. On the other hand, no shift in the frequential bandwidth was observed on these spectra, signifying a constancy in ankle stiffness over all conditions. Interestingly, the CNS does not really seem to gain from these reduced horizontal accelerations at the CG level since the CG(h) amplitudes are only slightly reduced. However, it is important to emphasize that the CP trajectories alone are not able to demonstrate any statistical trend. It can thus be hypothesized that, despite the fact that visual information is still unavailable, the proprioceptive cues nonetheless continue to play a minor role in the detection-correction process aimed at controlling body sway. Past studies on the physiology of eyes blinking have suggested the probability that the cerebellar cortex or brain stem structures (such as the reticular formation) are involved in these commands. Because of its dual facilitating-inhibiting function, the latter is indeed a fair candidate for modulating the descending command operating through the postural muscles. These data are of interest for the practician in order to assess with precision the role played by proprioceptive and visual cues in possible balance disfunctioning.

Published
2003

41. Impact of genomics on medicine.

Author

Zanders E

Subjects
Animals, Biotechnology trends, Drug Design, Humans, Pharmacogenetics, Protein Conformation, Proteins chemistry, Proteins genetics, Genomics, Medicine trends
Published
2002
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42. Cambridge Healthtech Institute's 5th Annual Conference: impact of genomics on medicine.

Author

Zanders ED

Subjects
DNA analysis, DNA chemistry, Drug Industry, Humans, Protein Biosynthesis, RNA, Messenger analysis, Genomics, Medicine
Abstract

The recent publications in Nature and Science by the Human Genome Consortium and Celera Genomics, respectively, while being landmark achievements in themselves, have also given pause for thought. A definitive catalogue of human genes is still not available but the broad picture of how humans compare with lower organisms at the genomic level is becoming clearer. The full impact of these findings on the practice of medicine is hard to predict, but research being conducted now, in the early years of the 21st century, will form the basis of future advances in the diagnosis and treatment of disease. Exactly what this will entail is the subject of intense debate, but there are some common starting points that were discussed at this meeting in Munich. The main theme to emerge was the need to move beyond the human genome sequence towards an understanding of proteins and their interactions in complex biological pathways, thereby increasing opportunities for drug discovery through the identification of new targets. The majority of the talks were therefore devoted to the description of technological advances in the analysis of gene and protein expression (and interaction) and in the use of various methods of gene deletion in order to validate individual proteins as drug targets. Perhaps it will still be a few years before it will be possible to report on the application of genomic analyses to routine medical practice at the first point of care for patients but when that happens, the research efforts described here will have been worthwhile.

Published
2001
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43. The end of the beginning for genomic medicine.

Author

Bailey D, Zanders E, and Dean P

Subjects
Animals, Biotechnology methods, Biotechnology trends, Computational Biology methods, Computational Biology trends, Drug Design, Evolution, Molecular, Genes, Human Genome Project, Humans, Proteins chemistry, Proteome, Drug Industry methods, Drug Industry trends, Genomics methods, Genomics trends
Published
2001
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44. Use of two-dimensional gel electrophoresis to measure changes in synovial fluid proteins from patients with rheumatoid arthritis treated with antibody to CD4.

Author

Smith MA, Bains SK, Betts JC, Choy EH, and Zanders ED

Subjects
Acute-Phase Proteins analysis, Antibodies, Monoclonal immunology, Antibodies, Monoclonal therapeutic use, Arthritis, Rheumatoid immunology, Arthritis, Rheumatoid therapy, Electrophoresis, Gel, Two-Dimensional methods, Feasibility Studies, Humans, Immunoglobulins immunology, Immunotherapy methods, Synovial Fluid immunology, Arthritis, Rheumatoid metabolism, CD4 Antigens immunology, Immunoglobulins therapeutic use, Proteins analysis, Synovial Fluid metabolism
Abstract

Synovial fluid proteins from microliter volumes of synovial fluid were resolved by two-dimensional polyacrylamide gel electrophoresis and detected by silver staining to investigate the feasibility of using two-dimensional (2D) electrophoresis in the clinical research setting and provide global disease information of disease progression. Several hundred proteins could be resolved as spots, many of which displayed the characteristic pattern of plasma-derived glycoproteins. The lowest level of detection was approximately 0.2 ng from a total of 50 microg of protein loaded. Most of the proteins could be identified on the basis of pI and molecular weight when compared with plasma protein maps on the World Wide Web. Unknown proteins were characterized by mass spectrometry of tryptic digests and by comparison with peptide databases. Synovial fluids from patients with rheumatoid arthritis were analyzed using this technique. Each subject received a fixed dose of antibody to CD4 as part of a phase II clinical trial to determine the efficacy of this immunosuppressive treatment in modifying disease activity. Synovial fluid was removed at day 0, followed by administration of antibody. Subsequent removal of synovial fluid and additional administration of antibody were carried out at different times thereafter. Changes in levels of acute-phase proteins were quantified by densitometry of silver-stained 2D polyacrylamide gels. Other parameters of disease progression such as serum C-reactive protein and physician's global assessment of clinical condition were used for comparison. In this way, changes in acute-phase proteins towards normal levels, as measured by 2D polyacrylamide gel electrophoresis, could be correlated with clinical improvement and conventional clinical chemistry measurements. Thus, the system can be used for quantitative analysis of protein expression in sites of autoimmune disease activity such as the synovial fluid of rheumatoid arthritis patients.

Published
2001
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45. Gene expression analysis as an aid to the identification of drug targets.

Author

Zanders ED

Subjects
Animals, Humans, Signal Transduction drug effects, Signal Transduction genetics, Gene Expression drug effects, Gene Expression genetics, Pharmacogenetics methods
Abstract

Many drug targets are components of complex signalling pathways, and in order to understand the true biological consequences of modulating these targets it is necessary to understand the biology of the system in great detail. Genomics research can contribute some of the tools to achieve this, for example through the use of cDNA microarrays. Since activation of signalling pathways leads to mRNA expression, microarray technology can be used to provide a detailed quantitative assessment of the consequences of this activation, often providing a completely new biological perspective on well established cellular systems. This review will discuss some of the results obtained using mRNA profiling of yeast and mammalian cells to analyse signalling pathways of relevance to inflammation and cancer, and will point towards the future applications of this exciting approach to drug target evaluation.

Published
2000
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46. Analysis of immune system gene expression in small rheumatoid arthritis biopsies using a combination of subtractive hybridization and high-density cDNA arrays.

Author

Zanders ED, Goulden MG, Kennedy TC, and Kempsell KE

Subjects
B-Lymphocytes immunology, Base Sequence, Case-Control Studies, DNA Primers genetics, Gene Expression, Humans, Macrophages immunology, Plasma Cells immunology, Synovial Membrane immunology, Arthritis, Rheumatoid genetics, Arthritis, Rheumatoid immunology, DNA, Complementary genetics, Genes, Immunoglobulin, Nucleic Acid Hybridization methods
Abstract

Subtractive hybridization of cDNAs generated from synovial RNA which had been isolated from patients with rheumatoid arthritis (RA) or normal controls was used in conjunction with high-density array hybridization to identify genes of immunological interest. The method was designed to detect gene expression in small needle biopsy specimens by means of a prior amplification of nanogram amounts of total RNA to full-length cDNA using PCR. The latter was cut with Rsa I, ligated with adapters, hybridized with unmodified driver cDNA, and subjected to suppression subtraction PCR. Differentially expressed products were cloned into E. coli and picked into 384 well plates. Inserts were obtained by PCR across the multiple cloning site, and the products arrayed at high density on nylon filters. The subtracted cDNAs were also labelled by random priming for use as probes for library screening. The libraries chosen were the subtracted one described above and a set of 45,000 ESTs from the I.M. A.G.E consortium. Clones showing positive hybridization were identified by sequence analysis and homology searching. The results showed that the subtracted hybridization approach could identify many gene fragments expressed at different levels, the most abundant being immunoglobulins and HLA-DR. The expression profile was characteristic of macrophage, B cell and plasma cell infiltration with evidence of interferon induction. In addition, a significant number of sequences without matches in the nucleotide databases were obtained, this demonstrates the utility of the method in finding novel gene fragments for further characterisation as potential members of the immune system. Although RA was studied here, the technology is applicable to any disease process even in cases where amounts of tissue may be limited.

Published
2000
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47. An AP-1 site in the promoter of the human IL-5R alpha gene is necessary for promoter activity in eosinophilic HL60 cells.

Author

Baltus B, van Dijk TB, Caldenhoven E, Zanders E, Raaijmakers JA, Lammers JW, Koenderman L, and de Groot RP

Subjects
Base Sequence, Cyclic AMP Response Element Modulator, Cyclic AMP Response Element-Binding Protein genetics, Cyclic AMP Response Element-Binding Protein metabolism, DNA Primers, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, HL-60 Cells, Humans, Mutagenesis, Site-Directed, Protein Binding, RNA, Messenger genetics, Receptors, Interleukin-5, Transcription Factor AP-1 genetics, Eosinophils metabolism, Promoter Regions, Genetic, Receptors, Interleukin genetics, Repressor Proteins, Transcription Factor AP-1 metabolism
Abstract

Interleukin-5 (IL-5) plays a crucial role in the proliferation, differentiation and activation of eosinophils. The IL-5 receptor is composed of an IL-5-specific alpha subunit, which is expressed by eosinophils and basophils, and a beta c-subunit shared with the receptors for IL-3 and GM-CSF. We identified an AP-1 element which is important for IL-5R alpha promoter activity in eosinophilic HL60 cells. The AP-1 site and the previously identified EOS1 site cooperate, since single mutation of either of the sites decreased promoter activity. We show that the AP-1 site of the IL-5R alpha promoter binds multiple proteins, including cJun, CREB, and CREM.

Published
1998
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48. Interleukin-5 receptor alpha chain mRNA is down-regulated by transforming growth factor beta 1.

Author

Zanders ED

Subjects
Base Sequence, Colforsin pharmacology, Cyclosporine pharmacology, Cytokines pharmacology, Dexamethasone pharmacology, Down-Regulation drug effects, Gene Expression Regulation, Leukemic drug effects, Growth Substances pharmacology, Humans, Leukemia, Erythroblastic, Acute, Molecular Sequence Data, Neoplasm Proteins biosynthesis, Neoplasm Proteins genetics, RNA, Messenger biosynthesis, RNA, Messenger genetics, RNA, Neoplasm biosynthesis, RNA, Neoplasm genetics, Receptors, Interleukin genetics, Receptors, Interleukin-5, Tetradecanoylphorbol Acetate pharmacology, Tretinoin pharmacology, Tumor Cells, Cultured, Receptors, Interleukin biosynthesis, Transforming Growth Factor beta pharmacology
Abstract

Interleukin-5 is a T cell-derived cytokine with actions restricted to the eosinophil/basophil lineage and a subset of murine B cells. High affinity receptors have been identified and shown to comprise an IL-5-specific alpha chain (IL-5R alpha) in association with a beta chain which is shared with the receptors for IL-3 and GM-CSF. Nothing is currently known of the factors which regulate the transcription and subsequent expression of the IL-5 receptor alpha chain; this study was undertaken, therefore, in order to identify agents which modulate IL-5R alpha mRNA levels, with the goal of understanding the regulation of this gene in vivo. The human IL-5-dependent erythroleukemia TF-1 was used as a source of mRNA which was analysed by northern blotting using a cDNA probe for IL-5R alpha. A range of cytokines and pharmacological agents were used in 20 hour cultures of TF-1 followed by northern analysis. Of these, only TGF-beta 1 and PMA showed any effect, which was a selective downregulation, although the PMA displayed some cytotoxicity over the long culture period. The remainder (interleukins 1 to 11, G-CSF, GM-CSF, LIF, SCF, erythropoetin, IFN-gamma, RANTES, MIP-1 alpha, FGF, EGF, PDGF, dexamethasone, forskolin, retinoic acid and cyclosporin A) failed to alter expression.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1994

49. Secondary immunoglobulin responses of BALB/c mice previously stimulated with goat anti-mouse IgD.

Author

Champion BR, Buckham S, Page K, Obray H, and Zanders ED

Subjects
Animals, Female, Goats, Immunoglobulin A biosynthesis, Immunoglobulin E biosynthesis, Immunoglobulin G biosynthesis, Interleukin-6 biosynthesis, Mice, Mice, Inbred BALB C, Antibodies, Anti-Idiotypic immunology, Immunoglobulin D immunology, Immunologic Memory
Abstract

Intravenous injection of goat antibodies to mouse IgD (GAMD) into BALB/c mice has been shown to induce vigorous T-cell dependent immunoglobulin responses, particularly of the IgG1 and IgE isotypes. We have confirmed these findings and show that IgA responses are also triggered in this model. Since the study of IgE regulation in allergic individuals is concerned with secondary and subsequent T- and B-cell responses, we boosted GAMD-primed mice with goat antibodies to IgE or IgA in an attempt to specifically retrigger IgE- and IgA-bearing memory B cells. However, we found that secondary IgG1, IgE and IgA production could be elicited equally well by either antibody preparation or by normal goat IgG (GIg). As with the primary response, GIg primed and boosted mice produced very low or undetectable IgG1, IgE and IgA responses. These data suggest that GAMD is very efficient at priming T cells specific for GIg epitopes and that once primed they can be readily re-triggered by GIg. Spleen cells taken 7 days after boosting GAMD-primed mice were found to spontaneously produce much higher levels of interleukin-6 (IL-6) in culture than cells from unboosted or GIg primed and boosted mice. In contrast to primary responses, where IgE levels return to background (less than 40 ng/ml) very quickly, circulating IgE levels in boosted mice initially declined before reaching a plateau level (approximately 1 microgram/ml) which was maintained for at least 148 days. IgG1 and IgA levels continued to fall over this same time period. Mice which had been primed (but not boosted) 10 months earlier were all found to have detectable IgE in their blood, despite the fact that following priming IgE becomes undetectable within 2-3 weeks. Since only a part of the IgE response was directed towards the antigen (GIg), these observations suggest the possibility that B cells initially primed to make IgE can be non-specifically retriggered in vivo.

Published
1991

50. Immunoregulation in the common marmoset, Calithrix jaccus: functional properties of T and B lymphocytes and their response to human interleukins 2 and 4.

Author

Quint DJ, Buckham SP, Bolton EJ, Solari R, Champion BR, and Zanders ED

Subjects
Animals, B-Lymphocytes drug effects, Cells, Cultured, Clone Cells, Female, Immunoglobulin G biosynthesis, Immunoglobulin M biosynthesis, Lymphocyte Activation, Lymphokines biosynthesis, Male, Recombinant Proteins pharmacology, T-Lymphocytes drug effects, B-Lymphocytes physiology, Callithrix immunology, Callitrichinae immunology, Interleukin-2 pharmacology, Interleukin-4 pharmacology, T-Lymphocytes physiology
Abstract

Non-human primates have been used to study immune function to a much lesser extent than readily available strains of inbred rodents. Nevertheless, in situations where it might be desirable, but impossible, to study human immune responses in vivo, lower primates could provide an acceptable alternative. In order to extent the knowledge of T- and B-lymphocyte function in lower primates, the common marmoset Callithrix jaccus was used as an experimental model. The functional similarities between this species and humans at the level of T-B co-operation in the antibody response were examined, and xenoreactive T-lymphocyte clones were obtained from marmoset spleen cells using Epstein-Barr virus (EBV)-transformed human B cells as stimulators. These clones could act as helper cells when co-cultured with human B lymphocytes, inducing the secretion of both IgM and IgG. Lymphokine production by mitogen-stimulated marmoset T-cell clones was also examined. Interleukins (IL) 2 and 4 activities were detected in clone supernatants using bioassays and interferon-gamma (IFN-gamma) was detected using a solid-phase ELISA system. However, SDS-PAGE analysis of biosynthetically labelled marmoset and human T-cell clone supernatant proteins revealed major differences between the soluble T-cell products of the two species. The proliferative responses of marmoset T and B cells to recombinant human IL-2 and IL-4 were also examined. Stimulation of [3H]thymidine uptake was detected in both T cell- and anti-IgM-stimulated B-cell cultures with both of the lymphokines. These results suggests that the key components of the antibody response are functionally conserved between lower primates and man and that the common marmoset may be useful as an in vivo model of immune function, particularly with regard to the role of interleukins such as IL-2 and IL-4.

Published
1990

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