ZIB

1

Electronic Resource

Effects of interleukin-2 (IL-2) on human plasma lipid, lipoprotein, and C-reactive protein (1990)

Rosenzweig, I. Bruce ; Wiebe, Donald A. ; Hank, Jacquelyn A. ; [et al.]

Springer

Biotherapy 2 (1990), S. 193-198

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ISSN: 1573-8280

Keywords: apolipoproteins ; C-reactive protein ; interferon ; interleukin-2

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract Six patients with confirmed malignant disease received four consecutive weekly cycles of human recombinant interleukin-2 (IL-2) 4 days/week, continuous iv. infusion, 3 × 106 U/m2/day. Plasma cholesterol decreased a mean of 7% within 24 hours after IL-2 infusion and decreased by 33% within 4 days. Plasma cholesterol was significantly lower than baseline concentration by day 21 (−21%), and day 25 (−41%) was significantly lower than day 21. Decreased plasma cholesterol was the result of decreased HDL and LDL cholesterol concentrations. Plasma triglyceride demonstrated a mean increase of 46% after 4 days of therapy and remained greater than baseline concentrations at all time points analyzed. Apolipoprotein AI and AII decreased concomitantly with HDL-cholesterol concentrations, whereas apolipoprotein B after an initial mean decrease of 17% during the first cycle was not significantly different from baseline during the fourth cycle. Apolipoprotein E and Lp(a) were not significantly affected by IL-2 treatment. Plasma C-reactive protein (CRP) increased by 79% within 24 hours of therapy, increased by 254% on day 4, then decreased to baseline concentrations by day 21 after 3 days off of IL-2. Day 25 CRP was elevated compared to both baseline and day 21 concentrations. IL-2 induced plasma lipoprotein changes may be due in part to the induction of interferon gamma.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02173519

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2

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BLT-esterase activity followingin vitro andin vivo activation of human lymphocytes with interleukin-2 (1991)

Cannon, Adria ; Hank, Jacquelyn A. ; Sondel, Paul M.

Springer

Biotherapy 3 (1991), S. 253-260

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ISSN: 1573-8280

Keywords: BLT-esterase ; cytotoxic cells ; immunotherapy ; interleukin-2 ; lymphokine-activated killer

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract BLT-esterase and cytolytic activity by humanin vitro andin vivo generated Lymphokine Activated Killer (LAK) cells were measured. Lysates made from peripheral blood lymphocytes (PBL) of both normal donors and cancer patients receiving IL-2 therapy were assayed for BLT-esterase activity in a spectro-photometric assay. Cytotoxicity of PBL was measured in a51Cr-release assay. Both BLT-esterase activity and cytotoxicity increased when normal-donor PBL were stimulatedin vitro with IL-2, with greater activities at higher IL-2 concentrations. The activities also increased over time, peaking at 6 days ofin vitro stimulation. Patient PBL had increased BLT-esterase and cytotoxic activities after 4 weeks ofin vivo IL-2 treatment. This association of BLT-esterase activity and cytotoxicity with IL-2 activation is consistent with the model that LAK cytotoxicity is mediated by secretion of BLT-esterase associated cytolytic granules. Lymphocytes obtained afterin vivo IL-2 treatment and cultured for 3-4 hours in IL-2 show markedly augmented cytotoxic activity but no increase in their BLT-esterase activity. These results indicate that the increased cytotoxicity observed after this brief pulse ofin vitro IL-2 followingin vivo IL-2 treatment must result from effects of IL-2 other than the production of more esterase-containing cytolytic granules.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02171689

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3

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Strategies for improving antitumor activity utilizing IL-2: Preclinical models and analysis of antitumor activity of lymphocytes from patients receiving IL-2 (1992)

Albertini, Mark R. ; Hank, Jacquelyn A. ; Sondel, Paul M.

Springer

Biotherapy 4 (1992), S. 189-198

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ISSN: 1573-8280

Keywords: cytokines ; immunotherapy ; interleukin-2 ; interleukin-2 receptors ; lymphokine activated killer cells

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Conclusions Considerable enthusiasm remains for the successful utilization of the immune system for the immunotherapy of human cancers. Immunotherapeutic maneuvers have been able to mediate impressive antitumor responses for some patients with advanced and refractory malignancies. Unfortunately, the number of patients who benefit from current immunotherapies is low, while the toxicity for many of the patients receiving these treatments is high. It is becoming quite clear that the development of successful immunotherapeutic strategies will involve a carefully chosen combination of immunotherapeutic modalities or of immunotherapy combined with either surgery, radiation therapy, or chemotherapy. The use of an IL-2 based regimen which is clinically tolerable and can provide significant immune activation continues to remain central to many of these treatment approaches. Preclinicalin vitro and animal model systems can evaluate promising treatment strategies, including combination approaches. As an effective immunotherapeutic approach will likely require use of a combination of biologically active agents, the scheduling of these therapies may have profound importance both for optimal antitumor responses as well as clinical tolerance.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF02174205

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4

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Analysis of T cell receptor β and γ genes from peripheral blood, regional lymph node and tumor-infiltrating lymphocyte clones from melanoma patients (1991)

Albertini, Mark R. ; Nicklas, Janice A. ; Chastenay, Bettejayne F. ; [et al.]

Springer

Cancer immunology immunotherapy 32 (1991), S. 325-330

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ISSN: 1432-0851

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary A total of 199 T cell clones from two melanoma patients were derived from progenitor T cells from recurrent melanoma, regional lymph nodes (either involved or uninvolved with malignancy) and peripheral blood by inoculating single cells directly into the wells of microtiter plates before in vitro expansion. The surface marker phenotype of most clones was CD4+CD8−, although some were CD4−CD8+. Genomic DNA prepared from all clones was analyzed by Southern blot hybridization using T cell receptor (TCR) β and γ gene probes, seeking clones with identical TCR gene rearrangement patterns as direct evidence for in vivo progenitor T cell clonal amplification. ProbingHindIII-digested DNA with TCRβ and TCRγ probes revealed several clones with identical TCR gene rearrangement patterns. These clones had subsequent probing ofBamHI-digested DNA with TCRβ and TCRγ probes, which showed all but 2 clones to have distinct rearrangement patterns. These analyses provide clear molecular evidence for in vivo polyclonal CD4+ T cell populations in each of several separate immune compartments in these patients.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01789051

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5

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Addition of interleukin-2in vitro augments detection of lymphokine-activated killer activity generatedin vivo (1990)

Hank, Jacquelyn A. ; Weil-Hillman, Gilda ; Surfus, Jean E. ; [et al.]

Springer

Cancer immunology immunotherapy 31 (1990), S. 53-59

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ISSN: 1432-0851

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary Thein vivo administration of repetitive weekly cycles of interleukin-2 (IL-2) to patients with cancer enhances the ability of freshly obtained peripheral blood lymphocytes (PBL) to lyse both the natural-killer(NK)-susceptible K562 and the NK-resistant Daudi targets. Lysis of both targets is significantly augmented by inclusion of IL-2 in the medium during the cytotoxicity assay. This boost is much greater for cells obtained following thein vivo IL-2 therapy than for cells obtained prior to the initiation of therapy or for cells from healthy control donors. In addition to direct lytic activity, the PBL obtained followingin vivo IL-2 show a rapid increase in lymphokine-activated killer (LAK) activity with more prolongedin vitro IL-2 exposure, indicating that LAK effectors primedin vivo respond with “secondary-like” kinetics to subsequent IL-2in vitro. Lymphocytes from healthy control individuals, cultured in IL-2 under conditions attempting to simulate thein vivo IL-2 exposure, function similarly to PBL obtained from patients following IL-2, in that low-level LAK activity was significantly boosted by inclusion of IL-2 during the cytotoxic assay and the cells also responded with secondary-like kinetics to subsequent IL-2in vitro. The augmentation of the LAK effect was also dependent on the dose of IL-2 added during the 4-h51Cr-release cytotoxicity assay, with higher doses of IL-2 having a more pronounced effect. While continuous infusion of IL-2 induces a greater cytotoxic potential per milliliter of blood obtained from patients, the peak serum IL-2 levels attained are greater with bolus IL-2 infusions. These pharmacokinetic results, together with the IL-2 dose dependence of LAK activity generatedin vivo shown in this report, suggest that a combination of treatment with bolus IL-2 infusions superimposed on continuous IL-2 infusion may transiently expose IL-2 dependent LAK cells, activatedin vivo, to higher concentrations of IL-2, facilitating theirin vivo cytotoxic potential.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01742496

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6

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Clinical and immunological effects of human recombinant interleukin-2 given by repetitive weekly infusion to normal dogs (1994)

Helfand, Stuart C. ; Soergel, Steve A. ; MacWilliams, Peter S. ; [et al.]

Springer

Cancer immunology immunotherapy 39 (1994), S. 84-92

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ISSN: 1432-0851

Keywords: Canine ; Cytotoxicity ; Interleukin-2 ; Invivo ; Infusion ; Lymphocyte

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract Four normal adult dogs received two consecutive weekly cycles of human recombinant interleukin-2 (IL-2) by continuous infusion for 4 days/week. The dose of IL-2 given to each dog was 3×106 units m−2 day−1. Toxicities consisted of mild vomiting, diarrhea, and lethargy to varying degrees in all the dogs. These side-effects were reversed when the treatment was discontinued. Fever, tachypnea, and weight gain were not seen. A marked lymphocytosis and eosinophilia developed in all dogs after completion of each course of IL-2 (resulting in a more than sevenfold increase in each cell type) and persisted for more than 1 month in some. Fresh peripheral blood lymphocytes (PBL) obtained during this lymphocytosis mediated enhanced in vitro lysis of a natural-killer-cell-sensitive canine tumor cell line (CTAC). The in vitro proliferative responses of these same PBL to IL-2 could be detected earlier, progressed faster, and involved more cells than PBL tested prior to IL-2 infusion. Thus, a relatively well-tolerated regime of IL-2 in dogs can induce dramatic increases in lymphocyte numbers and activation, which is associated with augmentation of their in vitro antitumor reactivity. The clinical effectiveness of this immunotherapeutic approach remains to be tested in tumor-bearing dogs where it could serve as a relevant large-animal model for immunotherapy of cancer with IL-2.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01525313

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7

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Clinical and immunological effects of human recombinant interleukin-2 given by repetitive weekly infusion to normal dogs (1994)

Helfand, Stuart C. ; Soergel, Steve A. ; MacWilliams, Peter S. ; [et al.]

Springer

Cancer immunology immunotherapy 39 (1994), S. 84-92

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ISSN: 1432-0851

Keywords: Key words: Canine – Cytotoxicity – Interleukin-2 – In vivo – Infusion – Lymphocyte

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract. Four normal adult dogs received two consecutive weekly cycles of human recombinant interleukin-2 (IL-2) by continuous infusion for 4 days/week. The dose of IL-2 given to each dog was 3 × 106 units m–2 day–1. Toxicities consisted of mild vomiting, diarrhea, and lethargy to varying degrees in all the dogs. These side-effects were reversed when the treatment was discontinued. Fever, tachypnea, and weight gain were not seen. A marked lymphocytosis and eosinophilia developed in all dogs after completion of each course of IL-2 (resulting in a more than sevenfold increase in each cell type) and persisted for more than 1 month in some. Fresh peripheral blood lymphocytes (PBL) obtained during this lymphocytosis mediated enhanced in vitro lysis of a natural-killer-cell-sensitive canine tumor cell line (CTAC). The in vitro proliferative responses of these same PBL to IL-2 could be detected earlier, progressed faster, and involved more cells than PBL tested prior to IL-2 infusion. Thus, a relatively well-tolerated regime of IL-2 in dogs can induce dramatic increases in lymphocyte numbers and activation, which is associated with augmentation of their in vitro antitumor reactivity. The clinical effectiveness of this immunotherapeutic approach remains to be tested in tumor-bearing dogs where it could serve as a relevant large-animal model for immunotherapy of cancer with IL-2.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF01525313

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8

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Transcription factor activation in lymphokine activated killer cells and lymphocytes from patients receiving IL-2 immunotherapy (1998)

Nicolet, Charles M. ; Surfus, Jean M. ; Hank, Jacquelyn A. ; [et al.]

Springer

Cancer immunology immunotherapy 46 (1998), S. 327-337

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ISSN: 1432-0851

Keywords: Key words Human ; Blood ; Cellular activation ; Transcription factors ; Human-clinical studies

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract Administration of the cytokine interleukin-2 (IL-2) can result in therapeutic benefits for individuals with renal cell carcinoma and melanoma. Here we report an analysis of the transcription factor families AP-1, Sp1, NF-κB, and signal transducers and activators of transcription (STAT) in cancer patients’ lymphocytes before and after IL-2 immunotherapy, as assessed by a gel-shift assay. An in vitro surrogate of IL-2 immunotherapy is the incubation of fresh peripheral blood mononuclear cells (PBMC) from healthy individuals in IL-2 for several days, resulting in the production of lymphokine-activated killer (LAK) activity in these cultures. One purpose of this study was to describe the profile of transcription factor activation in these different populations, and assess whether the patterns observed correlated with functional differences in these cells. Prior to in vivo IL-2 administration, the typical binding pattern of transcription factors in PBMC from patients resembled that seen in fresh PBMC from healthy individuals. Over a 3-week course of IL-2 therapy, in most patients the binding patterns of AP-1, Sp1, and NF-κB proteins changed to resemble those seen in PBMC activated by IL-2 in vitro. However, the cells obtained from IL-2-treated patients did not have low-level constitutive expression of STAT binding factors as did LAK cells. When these patient cells were further stimulated by IL-2 in vitro, additional differences in STAT induction patterns were noted. These data provide further information on the molecular events occurring in immune cells generated through in vivo and in vitro administration of IL-2, and further document that there is not a precise congruence between PBMC activated in vivo and in vitro by IL-2.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/s002620050494

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9

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Pharmacokinetics and stability of the ch14.18–interleukin-2 fusion protein in mice (1999)

Kendra, Kari ; Gan, Jacek ; Ricci, Melody ; [et al.]

Springer

Cancer immunology immunotherapy 48 (1999), S. 219-229

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ISSN: 1432-0851

Keywords: Key words Interleukin-2 ; Antitumor antibody ; Targetted immunotherapy ; Ganglioside

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Abstract The fusion protein formed from ch14.18 and interleukin-2 (ch14.18–IL-2), shown to exhibit antitumor efficacy in mouse models, consists of IL-2 genetically linked to each heavy chain of the ch14.18 chimeric anti-GD2 monoclonal antibody. The purpose of this study was to determine the pharmacokinetics of ch14.18–IL-2 in mice and assess its stability in murine serum. Following i.v. injection, the fusion protein was found to have a terminal half-life of 4.1 h. Detection of IL-2 following injection of the ch14.18–IL-2 fusion protein showed a similar half-life, indicating that the fusion protein prolongs the circulatory half-life of IL-2. Detection of human IgG1 following injection of ch14.18–IL-2 showed a terminal half-life of 26.9 h. These data suggested that the native fusion protein is being altered in vivo, resulting in a somewhat rapid loss of detectable IL-2, despite prolonged circulation of its immunoglobulin components. In vitro incubation of the ch14.18–IL-2 fusion protein in pooled mouse serum at 37 °C for 48 h resulted in a loss of its IL-2 component, as detected in enzyme-linked immunosorbent assay systems and in proliferation assays. Polyacrylamide gel electrophoresis and Western blot analysis of the fusion protein incubated in mouse serum at 37 °C indicated that the ch14.18–IL-2 is cleaved, resulting in a loss of the 67-kDa band (representing the IL-2 linked to the IgG1 heavy chain) and the detection of a band of more than 50 kDa, slightly heavier than the IgG1 heavy chain itself. This suggests that the fusion protein is being cleaved in vitro within the IL-2 portion of the molecule. These studies show that (1) ch14.18–IL-2 prolongs the circulatory half-life of IL-2 (compared to that of soluble IL-2) and (2) the in vivo clearance of the fusion protein occurs more rapidly than the clearance of the ch14.18 antibody itself, possibly reflecting in vivo cleavage within the IL-2 portion of the molecule, resulting in loss of IL-2 activity.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/s002620050569

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Clinical adoptive chemoimmunotherapy with allogeneic alloactivated HLA-haploidentical lymphocytes: controlled induction of graft-versus-host-reactions (1988)

Kohler, Peter C. ; Hank, Jacquelyn A. ; Minkoff, Deborah Z. ; [et al.]

Springer

Cancer immunology immunotherapy 26 (1988), S. 74-82

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ISSN: 1432-0851

Source: Springer Online Journal Archives 1860-2000

Topics: Medicine

Notes: Summary A total of 13 cancer patients were treated with Adoptive Chemoimmunotherapy (ACIT) using alloactivated HLA haploidentical lymphocytes. Donor lymphocytes were activated in vitro using a pool of irradiated allogeneic lymphocytes (MLC-cells) and some further expanded by culturing in T-cell growth factor (TCGF-cells). The first 6 patients received i.v. cyclophosphamide (CPM) followed 24 h later by escalating doses of MLC-cells, then 7 days later they received an infusion of TCGF-cells. Minimal toxicity was seen. The next 7 patients received CPM (800 mg/m2) and a combined MLC and TCGF-cell infusion (total cell dose ranged from 0.79×1010 to 2.26×1010). Of these 7 patients, 3 developed mild graft-versus-host reaction (GVHR) which resolved without treatment, and 2 patients had progressive GVHR which was arrested by methylprednisolone (2 mg/kg). Peripheral blood lymphocytes from these 2 patients, during the GVHR, had increased activated T-cells (OKT-10+ and OK-Ia+). In vitro expansion, in TCGF, of these activated T-cells enabled HLA typing to prove they were of donor origin. Only 1 clinical antitumor response was observed in the first 6 patients. The results of this study indicate that this form of ACIT can be given to patients with acceptable toxicity. Self-limited or easily controlled GVHR may be induced and primed donor cells persisting in the circulation are probably responsible. Further testing is required to determine whether the immune response induced by this form of ACIT may be therapeutically effective.

Type of Medium: Electronic Resource

URL: http://dx.doi.org/10.1007/BF00199851

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