|
|||||||||
|
|
|
|
|
|
|
|
|
|
|
Blood, Vol. 91 No. 11 (June 1), 1998:
pp. 4273-4281
By
From the Laboratory of Molecular Cytology, Department of Internal
Medicine, University of Innsbruck, Innsbruck, Austria.
B-chronic lymphocytic leukemia (B-CLL) is characterized by cellular
and humoral immune defects resulting in increased rates of infection
and disturbed immune surveillance against cancer cells as well as by
the expansion of slowly proliferating tumor cells. We found increased
Fas receptor (FasR) expression in peripheral blood CD4+
and CD8+ cells of B-CLL patients compared with the
equivalent cells of healthy donors. Although increased Fas receptor
expression was significant in both T-lymphocytic subsets, only
CD4+ cells from B-CLL patients underwent apoptosis after
treatment with the agonistic Fas antibody CH11. In CD4+
cells of B-CLL patients, the Fas-sensitivity also correlated with a
CD4+/CD8+ ratio below the lower threshold
of healthy individuals (<1.0). By contrast, FasR expression in the
CD19+ fraction of B-CLL patients was downregulated
compared with normal controls, and this was associated with an
insensitivity to CH11-induced apoptosis. The B-CLL cell line EHEB as
well as CD19+ cells from B-CLL patients constitutively
expressed Fas ligand (FasL). The FasL was functionally active, as the
B-CLL cell line as well as T-cell-depleted CD19+ B-CLL
fractions were able to kill target T-acute lymphatic leukemia (T-ALL)
cells in vitro. This effect was inhibited by the antagonistic FasR-antibody ZB4, the neutralizing anti-FasL monoclonal antibody (MoAb) NOK-2 or by transfection of the caspase inhibitor crmA. These
data point to the fact that expression of FasL on CD19+
B-CLL cells, together with enhanced susceptibility of
CD4+ T cells toward FasL-bearing effector cells, are
causally linked to the relative reduction of CD4+ cells
occurring during B-CLL progression. These findings could explain the
inversion of the ratio of CD4+/CD8+ cell
numbers, which may be causally linked to the immune deficiency observed
in these patients and to the expansion of the neoplastic clone in
B-CLL.
CHRONIC B-LYMPHOCYTIC leukemia (B-CLL)
represents a lymphoproliferative disease with clonal expansion of
immunologically immature CD5+ B cells. Clinically, the
disease is characterized by a distinct immune deficiency and by the
direct consequences of B-cell accumulation, ie, splenomegaly,
lymphadenopathy, bone marrow infiltration, and progressive
lymphocytosis.1 It has been speculated that an imbalance of
immunoregulatory T cells, mainly T-helper cells (CD4+)
and T suppressors (CD8+), is the main cause of the immune
deficiency.2,3 In fact, an inversion of the ratio of
CD4+/CD8+ cell numbers of <1.0 and a
deficiency in the function of the T-helper cells were reported by
several investigators.2-5 The pathologic T-cell
distribution together with the loss of T-cell activities were
correlated with the stage of disease and thought to be primarily
responsible for the impaired immunoregulation and the increased
frequencies of infectious episodes occurring in these
patients.2,6,7 However, the precise mechanisms responsible
for the imbalance of the T-cell subsets remain obscure. In partial
analogy to B-CLL, the primary features of human immunodeficiency virus
(HIV) disease are the prominent immune deficiency and a tight
correlation between an increasing frequency of infections on the one
hand and the inversion of the CD4+/CD8+
ratio8 and a progressive depletion of T
cells8,9 on the other. Recent data from HIV-infected
patients suggest the vital importance of the FAS receptor (FasR)/FAS
ligand (FasL) system in the pathogenesis of the above-mentioned
clinical and immunologic stigmata associated with this
disease.8-10
The FasR (CD95, APO-1) belongs to the tumor necrosis factor (TNF)
receptor supergene family, which, after binding of the specific ligand,
is capable of mediating cell death.11,12 In resting, naive
T cells, both the FasR and the FasL are expressed at low levels but are
upregulated upon activation by antigens by T-cell receptor (TCR)
signaling.13-15 The expression of FasR renders T cells
susceptible to activation-induced cell death (AICD) which, after
simultaneous upregulation of FasL, can proceed as "fratricide" and as "suicide" of the FasR+/FasL+
T cells.14,15 This cell death program leads to
the removal of high-risk cells, either remnants of an immune response
or self-reactive T cells in the periphery.16-18 In HIV
disease, the viral infection has been shown to lead to abnormal chronic
upregulation of FasR and FasL on both CD4+ and
CD8+ cells.8-10 In one of these studies,
different sensitivities of the purified CD4+ and
CD8+ cells to FasR-triggering MoAb CH11 were observed
leading in vitro to an inverted CD4+/CD8+
ratio.8
Besides expression on T cells, functional FasL expression has recently
been demonstrated on normal murine B cells stimulated with phorbol
12-myristate 13-acetate (PMA)/ionomycin.19 These FasL-bearing B lymphocytes were shown to kill FasR+ target
A20 B lymphoma cells in vitro.19 In the human system, we
recently reported the presence of functionally active FasL on
terminally differentiated neoplastic plasma cells.20 Our data on neoplastic plasma cells are part of accumulating evidence that
FasL-expressing tumor cells are able to kill target cells in
vitro.18 This mechanism of active killing has been
implicated in immune escape of tumor cells and by this mechanism
T-lymphocyte subsets involved in antitumor responses may be
inactivated.
These observations raise the question if the FasR/FasL system might be
involved in the pathophysiology of B-CLL, which is associated with
B-cell accumulation, immunodeficiency and inversion of the ratio of
CD4+/CD8+ cell numbers found in a high
percentage of B-CLL patients. Using a B-CLL cell line, native malignant
B cells as well as CD4+ and CD8+ T cells
derived from the peripheral blood of 33 patients, we studied the
interaction of B and T cells with the FasR/FasL system and its
contribution to the development of the disturbed homeostasis of
CD4+/CD8+ T cells in B-CLL.
Patients and Controls
Preparation of Peripheral Blood Lymphocytes
Cell Lines and Culture Conditions
Flow Cytometric Analysis FasL staining. Cells (0.5 × 106) were washed twice in phosphate-buffered saline (PBS), resuspended, and fixed in 1 mL paraformaldehyde (4%) for 15 minutes at 4°C. After an additional wash with PBS, the pellet was resuspended in chilled methanol (70%) and incubated for 5 minutes on ice. Cells were washed twice in PBS, incubated with 1 µg anti-FasL IgG1 MoAb (Transduction Laboratory, Lexington, KY) for 30 minutes at 4°C. Again, cells were washed twice with PBS, and incubated with 3 µL of fluorescein isothiocyanate (FITC)-labeled rabbit anti-mouse (DAKO, Copenhagen, Denmark) for 30 minutes at 4°C. The pellets were resuspended in 200 µL PBS and analyzed immediately. Negative controls were performed simultaneously using a mouse anti-human IgG1 MoAb (DAKO) instead of the anti-FasL MoAb. The FACS data were reported as the mean fluorescence intensity (MFI) ratios. This represents the MFI determined using the anti-FasL MoAb divided by the MFI obtained with the isotype negative control MoAbs. An MFI of >1.5 was considered positive. CD95 staining. Cells (0.5 × 106) were incubated with 10 µL FITC-conjugated anti-FasR IgG1 MoAb UB2 (Immunotech, Marseille, France) for 30 minutes at room temperature. Cells were washed twice with PBS, resuspended in 200 µL PBS, and analyzed immediately. Negative controls were performed simultaneously using an FITC-conjugated mouse anti-human IgG1 MoAb (DAKO) instead of the anti-FasR MoAb. The percentage of positive cells was calculated directly from the gated contour blot. Assay for FasR/FasL-Induced Cell Killing Target cell death of CEM-C7H2 vector control T-ALL cells resulting from their cocultivation with "effector" B-CLL cells was quantified by measuring target cell DNA fragmentation and loss using the JAM-test.20,24 For this purpose, T-ALL cells were incubated with 10 µCi/mL 3[H]-thymidine (Amersham, Buckinghamshire, UK) for 16 hours, washed three times with PBS, and resuspended in regular culture medium. A total of 100 µL of the T-cell suspension (2 × 104/mL) was cocultivated in 96-well plates with or without 100 µL of the relevant B-CLL cell suspension (2 × 105/mL). Where CD19+ B-CLL cells were used as effectors, PBMC of B-CLL patients were depleted of T cells by magnetic cell separation (Miltenyi Biotec, Sunnyvale, CA) according to the manufacturer's protocol. Briefly, PBMC were incubated with a cocktail of mouse anti-CD4 and anti-CD8 antibodies (DAKO), followed by incubation with anti-mouse antibodies bound to magnetic microbeads. T cells were magnetically trapped, resulting in a highly enriched fraction of CD19+ B cells (purity > 98%).
Assay of Apoptosis The binding of annexinV-FITC was used to follow phosphatidylserine exposition on early apoptotic cells.25 The staining was performed according to manufacturer's instructions. Briefly, 2.5 × 105 cells/mL were incubated with saturating concentrations of annexinV-FITC for 15 to 30 minutes at room temperature and immediately analyzed by flow cytometry.Data Presentation and Statistical Analysis Data of Figs 1-3 and 5A and B are depicted in box-blot and whiskers models. The box shows the median and the interquartile range of the data, whereas 25% of the data are within the range of a whisker in one direction. For statistical analysis of data, P values were assessed using a Fisher's PLSD test in the analysis of variance (ANOVA) program of StatView 5.1 (Abacus Concepts Inc, Berkeley, CA). Figure 4 comprises a flow cytometric profile of FasL expression on CD19+ B-CLL cells.
Expression of FasR Antigen on CD4+ and CD8+ Cells From Patients With B-CLL and Its Correlation With Fas-Induced Apoptosis To investigate the susceptibility of T-cell subsets toward Fas-induced apoptosis in B-CLL, we first determined the expression levels of the death receptor molecule FasR. FasR expression could be detected in a fraction of CD4+ cells (mean, 35%; range, 13% to 56%) and CD8+ cells (mean, 27%; range, 13% to 41%) from 20 healthy donors (Fig 1). In B-CLL patients (n = 33), a significantly higher number of FasR+ cells was found in the CD4+ (mean, 53%; range, 23% to 89%, P < .0001) and in the CD8+ subpopulations (mean, 45%; range, 22% to 79%, P < .0001) as compared with the normal equivalent cells (Fig 1).
Sensitivity of CD4+ Cells Toward Fas-Mediated Apoptosis
Correlates With CD4+/CD8+ Ratio in PBMC of
B-CLL Patients
FasL Expression in T-Lymphocyte Subsets of Normal Donors and B-CLL
Patients
Expression of FasR in B-CLL Lines and CD19+ Cells From
B-CLL Patients and Their Sensitivity to Fas-Induced Apoptosis
FasL Expression in B-CLL Lines and CD19+ B Lymphocytes of B-CLL Patients The expression of death-inducing FasL on the surface of cytotoxic cells or malignant tumor cells leads to target-cell killing in various tissues and cell types.18 To study the role of FasL expression on B cells in Fas-mediated apoptosis in the light of the enhanced sensitivity of CD4+ over CD8+ cells of B-CLL patients and over the equivalent cell fractions of healthy donors, we first analyzed surface FasL expression on the B-CLL cell line EHEB in flow cytometry which was found FasL positive with a MFI of 2.3 (mean of three experiments, data not shown). This result could also be confirmed in the CD19+ subpopulation of B-CLL patients, which showed a homogeneous staining profile of FasL in 27 of 30 patients (Table 2, Fig 4). A comparative study of CD19+ cells of B-CLL and normal donors showed no significant difference concerning FasL staining intensity (MFI of 2.4 ± .21 v 2.3 ± .1, P > .9; Table 2).Membrane-Bound FasL Antigen on B-CLL Cells Is Functional The expression of FasL on cytotoxic T lymphocytes (CTL) is reported to be sufficient for inducing cell death of FasR-bearing target cells.29 Using the JAM assay as a readout system, we examined whether FasL-expressing CD19+ B-CLL cells also exhibited cytolytic activity on the WT and crmA-transfected T-ALL cell line CEM-C7H2.20,22 These cells display features of activated T cells, such as expression of FasR and FasL14 and are susceptible to Fas-induced apoptosis by the agonistic FasR antibody CH11 or FasL+ effector cells.20 CEM-C7H2 cells carrying a vector control (VC) were prelabeled with [3H]thymidine and cocultivated for 72 hours with unlabeled EHEB cells resulting in a significant decrease in T-cell-specific [3H]thymidine content compared with untreated controls. This indicated the induction of DNA fragmentation and cell death in the target cells (Fig 5A). The effector/target ratio was tested over a broad range (2:1 to 20:1, data not shown) with T-cell killing most effective at the E/T ratio 10:1. Preincubation of target cells with the antagonistic FasR-antibody ZB4 (0.25 µg/mL) partially protected CEM-C7H2 cells from being killed by B-CLL cells (mean inhibition, 30% [P < .0001]; Fig 5A). crmA-transfected CEM-C7H2 cells were resistant to CH11 MoAb20,28 (and results not shown), reflecting the inhibition of caspase-8, which is involved in Fas-induced signaling.23,30 This target cell subclone (CRM) exhibited a high resistance to the killing mediated by the FasL-positive effector cell line EHEB (mean inhibition, 66%; P < .0001; Fig 5A). As a control experiment, a FasR B cell line
U26620 was used as a target for the FasL+ EHEB
cell line in a JAM assay. No killing of the FasR negative target cells
could be observed (mean percentage of apoptotic cells, 8%; Fig 5A),
thus arguing against an FasL-independent mechanism of killing in these
experiments.
This study showed a pronounced increase of FasR+ cells in CD4+ and CD8+ T-cell fractions of B-CLL patients in comparison to healthy controls (Fig 1). This was associated with a sensitivity of the CD4+ cell fraction toward Fas-mediated apoptosis in vitro (Fig 2a). In the same experimental setting, we found that the CD8+ fraction, despite having a similarly high percentage of FasR+ cells, proved far less sensitive to Fas-mediated cell death triggered by CH11 MoAb in the time frame investigated (after 24 hours, Fig 2A; after up to 7 days, data not shown). By contrast, although FasR expression could be found in a mean of 35% of the CD4+ and 27% of the CD8+ fraction of cells of healthy volunteers, neither of the T-cell subsets were susceptible to cell death by the same treatment with CH11 MoAb (Fig 2B). These results in healthy controls are in line with other investigations in which FasR expression was determined in a mean of about 30% in both CD4+ and CD8+ T cells of healthy donors, which nevertheless remained resistant to Fas-mediated apoptosis.8,9
Submitted October 14, 1997;
accepted January 24, 1998.
1. Cheson BD, Bennett JM, Rai KR, Grever MR, Kay NE, Schiffer CA, Oken MM, Keating MJ, Boldt DH, Kempin SJ, Foon KA: Guidelines for clinical protocols for chronic lymphocytic leukemia: Recommendations of the National Cancer Institute-sponsored working group. Am J Hematol 29:152, 1988[Medline] [Order article via Infotrieve] 2. Herrmann F, Lochner A, Philippen H, Jauer B, Ruehl H: Imbalance of T-cell subpopulations in patients with chronic leukemia of the B cell type. Clin Exp Immunol 49:157, 1982[Medline] [Order article via Infotrieve] 3. Platsoucas CD, Galinski M, Kempin S, Reich L, Clarkson B, Good RA: Abnormal T-lymphocyte subpopulations in patients with B cell chronic lymphocytic leukemia: An analysis by monoclonal antibody. J Immunol 129:2305, 1982[Medline] [Order article via Infotrieve]
4.
Kay NE:
Abnormal T-cell subpopulation function in CLL: Excessive suppressor and deficient helper (T) activity with respect to B-cell proliferation.
Blood
57:418,
1981
5.
Chiorazzi N,
Fu SM,
Montazeri G,
Kunkel HG,
Rai K,
Gee T:
T-cell helper defect in patients with chronic lymphocytic leukemia.
J Immunol
122:1087,
1979
6.
Peller S,
Kaufman S:
Decreased CD45RA T-cells in B-cell chronic lymphatic leukemia patients: Correlation with disease stage.
Blood
78:1569,
1991
7.
Tötterman TH,
Carlsson M,
Simonsson B,
Bengtsson M,
Nilsson K:
T-cell activation and subset patterns are altered in B-CLL and correlate with the stage of the disease.
Blood
74:786,
1989
8.
Sloand EM,
Young NS,
Kumar P,
Weichold FF,
Sato T,
Maciejewski JP:
Role of Fas ligand and receptor in the mechanism of T-cell depletion in acquired immunodeficiency syndrome: Effect on CD4+ lymphocyte depletion and human immunodeficiency virus replication.
Blood
89:1357,
1997
9.
Estaquier J,
Tanaka M,
Suda T,
Nagata S,
Golstein P,
Ameisen JC:
Fas-mediated apoptosis of CD4+ and CD8+ T-cells from human immunodeficiency virus-infected persons: Differential in vitro preventive effect of cytokines and protease antagonists.
Blood
87:4959,
1996 10. Aries SP, Schaaf B, Muller C, Dennin RH, Dalhoff K: Fas(CD95) expression on CD4+ T-cells from HIV-infected patients increases with disease progression. J Mol Med 73:591, 1995[Medline] [Order article via Infotrieve] 11. Itoh N, Yonehara S, Ishii A, Yonehara M, Mizushima S, Sameshima M, Hase A, Seto Y, Nagata S: The polypeptide encoded by the cDNA for human cell surface antigen Fas can mediate apoptosis. Cell 66:233, 1991[Medline] [Order article via Infotrieve]
12.
Nagata S,
Golstein P:
The Fas death factor.
Science
267:1449,
1995 13. Latinis KM, Carr LL, Peterson EJ, Norian LA, Eliason SL, Koretzky GA: Regulation of CD95 (Fas) ligand expression by TCR-mediated signaling events. J Immunol 158:4602, 1997[Abstract] 14. Ju ST, Panka DJ, Cui H, Ettinger R, el Khatib M, Sherr DH, Stanger BZ, Marshak Rothstein A: Fas(CD95)/FasL interactions required for programmed cell death after T-cell activation. Nature 373:444, 1995[Medline] [Order article via Infotrieve] 15. Brunner T, Mogil RJ, LaFace D, Yoo NJ, Mahboubi A, Echeverri F, Martin SJ, Force WR, Lynch DH, Ware CF, Green DR: Cell-autonomous Fas (CD95)/Fas-ligand interaction mediates activation-induced apoptosis in T-cell hybridomas. Nature 373:441, 1995[Medline] [Order article via Infotrieve] 16. Lynch DH, Ramsdell F, Alderson MR: Fas and FasL in the homeostatic regulation of immune responses. Immunol Today 16:569, 1995[Medline] [Order article via Infotrieve] 17. Hahn S, Gehri R, Erb P: Mechanism and biological significance of CD4-mediated cytotoxicity. Immunol Rev 146:57, 1995[Medline] [Order article via Infotrieve] 18. Walker PR, Saas P, Dietrich PY: Role of Fas ligand (CD95L) in immune escape: The tumor cell strikes back. J Immunol 158:4521, 1997[Abstract] 19. Hahne M, Renno T, Schroeter M, Irmler M, French L, Bornard T, MacDonald HR, Tschopp J: Activated B cells express functional Fas ligand. Eur J Immunol 26:721, 1996[Medline] [Order article via Infotrieve]
20.
Villunger A,
Egle A,
Marschitz M,
Kos M,
Boeck G,
Ludwig H,
Geley S,
Kofler R,
Greil R:
Constitutive expression of Fas (Apo-1/CD95) ligand on multiple myeloma cells: A potential mechanism of tumor-induced suppression of immune surveillance.
Blood
90:12,
1997 21. Saltman D, Bansal NS, Ross FM, Ross JA, Turner G, Guy K: Establishment of a karyotypically normal B-chronic lymphocytic leukemia cell line; evidence of leukemic origin by immunoglobulin gene rearrangement. Leuk Res 14:381, 1990[Medline] [Order article via Infotrieve]
22.
Strasser-Wozak E,
Hattmannstorfer R,
Hala M,
Hartmann B,
Fiegl M,
Geley S,
Kofler R:
Splice site mutations in the glucocorticoid receptor gene causes resistance to GC-induced apoptosis in a human acute leukemia cell line.
Cancer Res
55:348,
1995 23. Enari M, Hug H, Nagata S: Involvement of an ICE-like protease in Fas-mediated apoptosis. Nature 375:78, 1995[Medline] [Order article via Infotrieve] 24. Matzinger P: The JAM test. A simple assay for DNA fragmentation and cell death. J Immunol Methods 145:185, 1991[Medline] [Order article via Infotrieve]
25.
Martin SJ,
Reutelingsperger CP,
McGahon AJ,
Rader JA,
van Schie RC,
LaFace DM,
Green DR:
Early redistribution of plasma membrane phosphatidylserine is a general feature of apoptosis regardless of the initiating stimulus: Inhibition by overexpression of Bcl-2 and Abl.
J Exp Med
182:1545,
1995
26.
Yonehara S,
Shii A,
Yonehara M:
A cell-killing monoclonal antibody (anti-Fas) to a cell surface antigen co-downregulated with the receptor of tumor necrosis factor.
J Exp Med
169:1747,
1989 27. Amadori A, Zamarchi R, De Silvestro G, Forza G, Cavatton G, Danieli GA, Clementi M, Chieco-Bianchi L: Genetic control of the CD4/CD8 T-cell ratio in humans. Nature Med 1:1279, 1995[Medline] [Order article via Infotrieve]
28.
Villunger A,
Egle A,
Kos M,
Hartmann BL,
Geley S,
Kofler R,
Greil R:
Drug-induced apoptosis is associated with enhanced Fas (Apo-1/CD95) ligand expression but occurs independently of Fas (Apo-1/CD95) signaling in human T-acute lymphatic leukemia cells.
Cancer Res
57:3331,
1997 29. Suda T, Takahashi T, Golstein P, Nagata S: Molecular cloning and expression of the Fas ligand, a novel member of the tumor necrosis factor family. Cell 75:1169, 1993[Medline] [Order article via Infotrieve] 30. Muzio M, Chinnaiyan AM, Kischkel FC, O'Rourke K, Shevchenko A, Ni J, Scaffidi C, Bretz JD, Zhang M, Gentz R, Mann M, Krammer PH, Peter ME, Dixit VM: FLICE, a novel FADD-homologous ICE/CED-3-like protease, is recruited to the CD95 (Fas/APO-1) death-inducing complex. Cell 85:817, 1996[Medline] [Order article via Infotrieve]
31.
Oyaizu N,
McCloskey T,
Than S,
Hu R,
Kalyanaraman VS,
Pahwa S:
Cross-linking of CD4 molecules upregulates Fas antigen expression in lymphocytes by inducing interferon- 32. Sieg S, Huang Y, Kaplan D: Viral regulation of CD95 expression and apoptosis in T-lymphocytes. J Immunol 159:1192, 1997[Abstract] 33. Amasaki Y, Kobayashi S, Takeda T, Ogura N, Jodo S, Nakabayashi T, Tsutsumi A, Fujiskaku A, Koike T: Up-regulated expression of Fas antigen (CD95) by peripheral naive and memory T-cell subsets in patients with systemic lupus erythematosus (SLE): A possible mechanism for lymphopenia. Clin Exp Immunol 99:245, 1995[Medline] [Order article via Infotrieve]
34.
di Celle PF,
Carbone A,
Marchis D,
Zhou D,
Sozzani S,
Zupo S,
Pini M,
Mantovani A,
Foa R:
Cytokine gene expression in B-cell chronic lymphocytic leukemia: Evidence of constitutive interleukin-8 (IL-8) mRNA expression and secretion of biologically active IL-8 protein.
Blood
84:220,
1994
35.
Trentin L,
Zambello R,
Agostini C,
Enthammer C,
Cerutti A,
Adami F,
Zamboni S,
Semenzato G:
Expression and regulation of tumor necrosis factor, interleukin-2 and hematopoietic growth factor receptors in B-cell chronic lymphocytic leukemia.
Blood
84:4249,
1994
36.
Giordano C,
Stassi G,
De Maria R,
Todaro M,
Richiusa P,
Papoff G,
Ruberti G,
Bagnasco M,
Testi R,
Galluzzo A:
Potential involvement of Fas and its ligand in the pathogenesis of Hashimoto's thyroiditis.
Science
275:960,
1997
37.
Alderson MR,
Armitage RJ,
Maraskovsky E,
Tough TW,
Roux E,
Schooley K,
Ramsdell F,
Lynch DH:
Fas transduced activation signals in normal human T-lymphocytes.
J Exp Med
178:2231,
1993 38. Miyawaki T, Uehara T, Nibu R, Tsuji T, Yachie A, Yonehara S, Taniguchi N: Differential expression of apoptosis-related antigen on lymphocyte subpopulations in human peripheral blood. J Immunol 149:3753, 1992[Abstract] 39. Rathmell JC, Townsend SE, Xu JC, Flavell RA, Goodnow CC: Expansion or elimination of B cells in vivo: Dual roles for CD-40 and Fas ligands modulated by the B-cell antigen receptor. Cell 87:319, 1996[Medline] [Order article via Infotrieve] 40. Rothstein TL, Wang JK, Panka DJ, Foote LC, Wang Z, Stanger B, Cui H, Ju ST, Marshak Rothstein A: Protection against Fas-dependent Th1-mediated apoptosis by antigen receptor engagement in B cells. Nature 374:163, 1995[Medline] [Order article via Infotrieve] 41. Foote LC, Howard RG, Marshak-Rothstein A, Rothstein TL: IL-4 induces Fas-resistance in B cells. J Immunol 157:2749, 1996[Abstract]
42.
Hashimoto F,
Oyaizu N,
Kalyanaraman VS,
Pahwa S:
Modulation of Bcl-2 protein by CD4 cross-linking: A possible mechanism for lymphocyte apoptosis in human immunodeficiency virus infection and for rescue of apoptosis by interleukin-2.
Blood
90:745,
1997
© 1998 by The American Society of Hematology.
| |||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
 |
|
 |
|
  J. Greiner, L. Bullinger, B.-a. Guinn, H. Dohner, and M. Schmitt Leukemia-Associated Antigens Are Critical for the Proliferation of Acute Myeloid Leukemia Cells Clin. Cancer Res., November 15, 2008; 14(22): 7161 - 7166. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 A. Anichini, R. Mortarini, L. Romagnoli, P. Baldassari, A. Cabras, C. Carlo-Stella, A. M. Gianni, and M. Di Nicola Skewed T-cell differentiation in patients with indolent non-Hodgkin lymphoma reversed by ex vivo T-cell culture with {gamma}c cytokines Blood, January 15, 2006; 107(2): 602 - 609. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 R. Greil, G. Anether, K. Johrer, and I. Tinhofer Tracking death dealing by Fas and TRAIL in lymphatic neoplastic disorders: pathways, targets, and therapeutic tools J. Leukoc. Biol., September 1, 2003; 74(3): 311 - 330. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
S.-i. Fujii, K. Shimizu, F. Koji, and F. Kawano Malignant counterpart of myeloid dendritic cell (DC) belonging to acute myelogenous leukemia (AML) exhibits a dichotomous immunoregulatory potential J. Leukoc. Biol., January 1, 2003; 73(1): 82 - 90. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 K. Rosen, W. Shi, B. Calabretta, and J. Filmus Cell Detachment Triggers p38 Mitogen-activated Protein Kinase-dependent Overexpression of Fas Ligand. A NOVEL MECHANISM OF ANOIKIS OF INTESTINAL EPITHELIAL CELLS J. Biol. Chem., November 22, 2002; 277(48): 46123 - 46130. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
A. M. Krackhardt, S. Harig, M. Witzens, R. Broderick, P. Barrett, and J. G. Gribben T-cell responses against chronic lymphocytic leukemia cells: implications for immunotherapy Blood, June 17, 2002; 100(1): 167 - 173. [Abstract] [Full Text] [PDF]
|
|
|
|
|
|
G. Anether, I. Marschitz, I. Tinhofer, and R. Greil Interleukin-15 as a potential costimulatory cytokine in CD154 gene therapy of chronic lymphocytic leukemia Blood, January 15, 2002; 99(2): 722 - 723. [Full Text] [PDF]
|
|
|
|
|
|
A. Sampalo, G. Navas, F. Medina, C. Segundo, C. Camara, and J. A. Brieva Chronic lymphocytic leukemia B cells inhibit spontaneous Ig production by autologous bone marrow cells: role of CD95-CD95L interaction Blood, November 1, 2000; 96(9): 3168 - 3174. [Abstract] [Full Text] [PDF]
|
|
|
|
 |
|
 H. L. Maecker, C. Koumenis, and A. J. Giaccia p53 Promotes Selection for Fas-mediated Apoptotic Resistance Cancer Res., August 1, 2000; 60(16): 4638 - 4644. [Abstract] [Full Text]
|
|
|
|
 |
|
 I TINHOFER, H WYKYPIEL, I MARSCHITZ, T HENN, R GREIL;, M W BENNETT, J O'CONNELL, D ROCHE, C BRADY, J KELLY, et al. Gastric cancer cell lines lack Fas ligand (FasL) expression but kill T cells via a FasL independent pathway • Reply Gut, May 1, 2000; 46(5): 738 - 740. [Full Text] [PDF]
|
|
|
|
 |
|
 B. Drenou, V. Blancheteau, D. H. Burgess, R. Fauchet, D. J. Charron, and N. A. Mooney A Caspase-Independent Pathway of MHC Class II Antigen-Mediated Apoptosis of Human B Lymphocytes J. Immunol., October 15, 1999; 163(8): 4115 - 4124. [Abstract] [Full Text] [PDF]
|
|
| ||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||||
 |
 |
 |
|||||||
 |
 |
 |
 |
 |
 |
 |
 |
||
| Copyright © 1998 by American Society of Hematology Online ISSN: 1528-0020 | |||||||||
Abstract
Introduction
Abstract
-scintillation counter. The reduction in
incorporated radioactivity was used to calculate the percentage of
specific target cell killing:
![[(cpm<SUB>untreated cells</SUB> − cpm<SUB>cocultured cells</SUB>)/cpm<SUB>untreated cells</SUB> × 100]](/content/vol91/issue11/fulltext/4273/img001.gif)
). For blocking experiments,
crmA-expressing CEM-C7H2 cells (CRM) were used as target cells.
Alternatively, the labeled T-cells (VC) were coincubated with 0.25 µg/mL of the FasR blocking ZB4 MoAb. In a control experiment the
FasR- neoplastic B-cell line U266 was used as a target
(
). Cocultivation of cells was performed for 72 hours at 37°C.
The reduction of DNA-incorporated radioactivity was used to calculate
the percentages of B-CLL-mediated target cell death (n = 12) and is
presented in a box-blot and whiskers model. Statistical analysis of the
blocking experiments showed the following: specific killing by EHEB:
30% mean inhibition by ZB4 (P < .0001), 66% mean inhibition
by crmA expression (P < .0001). (B) CEM-C7H2 T-ALL cells are
eliminated by CD19+ cells of B-CLL patients through the
Fas/FasL pathway. PBMC of 5 B-CLL patients were depleted of T cells by
magnetic cell separation. The resulting CD19+ B-cell
fractions (purity > 98%) were cocultivated with
[3H]-thymidine-prelabeled CEM-C7H2 target cells for 72 hours at 37°C in a effector/target ratio of 10:1 (four replicates).
The reduction of DNA-incorporated radioactivity in the target cells was
used to calculate specific target cell killing by CD19+
B-CLL cells, which was blocked by preincubation with the antagonistic anti-FasR MoAb ZB4 (0.25 mg/mL, 
) or the inhibitory anti-FasL MoAb
NOK-2 (0.75 mg/mL, 
). Results of the statistical analysis: 44% mean
inhibition by ZB4 MoAb (.0001 < P < .002), 74% mean
inhibition by NOK-2 MoAb (P < .0001).
or
interferon-
.