I. Introduction
Recent success with mAbs as cancer therapeutics (Bell,
2002; Boye et al, 2003; Mendelsohn, 2003; Zelenetz, 2003) has renewed the
attention to the anti-cancer role of humoral immunity, including natural
humoral immunity. Natural anti-tumor antibodies are common for healthy
individuals (Colnaghi et al, 1982), and experimental in vivo data on their strong tumor-suppressive activity (David et
al, 1996) support their possible role in tumor immunosurveillance. Such
antibodies usually belong to the IgM isotype (Brandlein et al, 2003), which
might limit their infiltration into solid tumors (compared to smaller IgGs) and
restrict their anti-tumor effector function since no antibody-dependent
cellular cytotoxicity (ADCC) is known for IgMs. In addition, the applicability
of natural anticancer antibodies may be limited by their restricted specificity
against only certain tumor types (Cote et al, 1983). We have identified a
subset of natural IgG class antibodies capable of binding to the surface of a
broad spectrum of various cancer cells but not normal cells (Iakoubov,
Torchilin, 1997). These antibodies are natural antinuclear autoantibodies
(ANAs) that are present in a proportion of healthy rodents and humans,
especially in the aged (Xavier et al, 1995). Our hypothesis that these ANAs
participate in tumor immunosurveillance (Torchilin et al, 2001) was strongly
supported by the results of pre-clinical in
vivo experiments with mAb 2C5, a monoclonal tumor cell surface-reactive
nucleosome (NS)-specific ANA of IgG2a isotype obtained from a non-immunized
healthy aged Balb/c mouse. Within syngeneic mouse models, mAb 2C5 suppressed
the growth of EL4 T lymphoma and led to a prolonged survival time in B16
melanoma-bearing mice (Iakoubov and Torchilin, 1997). Existing data on the
tumor reactivity and anti-tumor properties of certain ANAs related to autoimmune
pathology or induced by immunization also favor this hypothesis (Brinkman et
al, 1993; Johnson, Shin, 1983; Sorace, Johnson, 1990). Numerous additional data
supporting the hypothesis on ANAsÕ role in tumor immunosurveillance have been
reviewed recently (Torchilin et al, 2003).
ADCC was considered as a most probable in vivo mechanism for mAb 2C5 anti-tumor
activity because of significant ADCC effect of this antibody in vitro (Iakoubov and Torchilin, 1997).
Though in vitro experiments did
reveal neither complement-mediated cytotoxicity, nor direct inhibition of tumor
cell proliferation, some additional mechanisms might be involved in vivo. By forming immune complexes
with free NSs in the circulation, mAb 2C5 and similar antibodies might induce
the enhanced release of inflammatory cytokines and proteolytic enzymes from
certain immune cells (Lucisana and Mantovani, 1984), as well as toll
receptor-involving events (Leadbetter et al, 2002), and/or empowerment of
dendritic cell (Schuurhuis et al, 2002).
The ability to recognize tumor but not normal cells
was observed for mAb 2C5 and another similarly obtained ANA, mAb 1G3. Both mAbs
demonstrated NS-restricted specificity. Thus, tumor cell surface-bound NSs
(supramolecular constituents of nuclear material consisting of
well-characterized individual monoNS composed of DNA and four pairs of histones
arranged in a characteristic pattern) were proposed to be their target on tumor
cells (Iakoubov, Torchilin, 1997). The binding of extracellular NSs to tumor
cell surface might be mediated by specific NS receptors that have been
repeatedly reported by several investigators to be present on the surface of
tumor cells (Jacob et al, 1989; Koutouzov et al, 1996; Seddiki et al, 2001). As
for the origin of tumor cell-bound NSs, extracellular NSs were found in tumor
cell cultures (Bell, Morrison, 1991) and in patients with tumors (Le
Lann-Terrisse et al, 1994), where they arise from apoptotic tumor cells present
in every in vivo developing tumor
(Wyllie, 1993). In cell culture experiments, NSs released from apoptotic S49 T
lymphoma cells after sub-optimal dexamethasone treatment were able to attach to
the surface of surviving cells. This was accompanied by a 50-fold increase in
monoclonal ANA 2C5 binding to these cells (Iakoubov and Torchilin, 1998).
Elevated free extracellular nucleochromatin has also been observed under other,
non-cancerous conditions accompanied by massive apoptotic death, such as lupus
erythematosis and AIDS (Licht et al, 2001). It is especially important, that
NSs are exposed on the cell surface of apoptotic cells (Radic et al, 2004).
Functionally, extracellular chromatin fragments have
been shown to inhibit the tumor cell killing by NK cells in vitro (Le Lann-Terisse et al, 1994, 1997). Such data allow considering
the NS release by dying tumor cells as a tumor self-defense mechanism that
protects the surviving tumor cells from host immune attack. In this case, the
increased production of NS-specific cytotoxic autoantibodies by a tumor-bearing
organism may be contemplated a response that acts to overcome the tumor
self-defense. The data demonstrating a prolonged time to disease progression
and an increased survival rate in cancer patients with elevated serum ANAs
(Blaes et al, 2000; Syrigos et al, 2000), and a higher remission rate in
chronic myelogenous leukemia patients who develop autoimmune phenomena (known
to be accompanied with a rise in ANAs) as a result of alpha-interferon therapy
vs those who do not (Sacchi et al, 1995) support a possibility of anti-tumor
activity of ANAs. Here, we present the first experimental data on strong
anti-tumor activity of mAb 2C5 against diverse human tumors in in vivo models.
In addition, the specificity
of mAb 2C5 and similar antibodies against a broad variety of tumors is a
prerequisite for their broad applicability as vehicles for targeting different
therapeutic and diagnostic agents to various tumors (Torchilin et al, 2003).
Supporting data on mAb 2C5Õs ability for intratumoral accumulation are also
presented.
II. Materials
and methods
A. Materials
All cell culture media,
heat-inactivated fetal bovine serum, and other cell culture reagents were
obtained from Cellgro (Herndon, VA). Isotype-matching control antibody UPC10
and fluorescein-conjugated goat anti-mouse antibody were purchased from ICN
Pharmaceuticals, Inc. (Cosa Mesa, CA). Diethylene triamine pentaacetic acid
anhydride (DTPA) for radiolabeling mAb 2C5 with 111In and all other
chemicals and buffer solution components were obtained from Sigma (St. Louis,
MO) and were of analytical grade. 111In with specific radioactivity
of 395 Ci/mg was from Perkin-Elmer (Boston, MA).
B.
Monoclonal antinuclear autoantibody 2C5 (mAb 2C5)
mAb 2C5 [IgG2a] (Iakoubov,
Torchilin, 1997) was purified from the supernatant of 2C5 hybridoma cells grown
in the CM10 culture medium by using a standard saturated ammonium sulfate
precipitation and affinity chromatography on a protein G column (Exalpha
Biologicals, Inc., Watertown, MA). Non-reducing SDS-PAGE of the purified
antibody (Laemmli, 1970), and ELISA with purified monoNSs (Li et al, 1995) were
performed to test mAb 2C5 purity and immunoreactivity. The purified antibody
was stored at -80¡C as a 5 mg/ml solution.
To label
the mAb 2C5 with 111In, it was first modified with chelating
residues DTPA and loaded with 111In by transchelation from the 111In-citrate
complex (Samokhin et al, 2001).
C.
Determination of the dissociation constant KD of monoNSs-mAb 2C5
complexes in solution by ELISA (Friguet et al, 1985)
The referenced protocol
includes the incubation of the antigen [monoNSs purified as in (Li et al,
1995), in this particular case] at various concentrations with mAb 2C5 at
constant concentration until equilibrium is reached and subsequent
determination of the free antibody concentration by an indirect ELISA. Samples
of monoNSs at various concentrations (0.016 - 16 mg/ml) were mixed with the
constant amount of antibody (1 mg/ml) in TBS, 2mM EDTA, pH
7.5, supplemented with 10 mg/ml BSA. After a 15 h incubation at 20¡C, 100ml of each mixture was
transferred and incubated for 30 min at 20¡C into the wells of a
microtiter plate coated with monoNSs [100 ml per well, at 10 mg/ml in TBST-Cas (TBS
containing 0.05% w/v Tween-20 and 2 mg/ml casein), pH 7.5, for 1 h at 20¡C]. After washing with TBS
supplemented with 0.05% Tween 20, the wells were incubated for 1 h at room
temperature with 100 ml of 1:5000 diluted goat
anti-mouse IgG peroxidase conjugate (ICN Biomedicals Inc., OH) in TBST-Cas.
After incubation, the wells were washed three times with 200 ml of TBST and each well was
incubated with 100ml of enhanced K-blue¨ TMB peroxidase substrate
(Neogen Corporation, KY) for 15 min. Finally, the plate was read at a dual
wavelength of 620 nm with the reference filter at 492 nm using a Labsystems
Multiskan MCC/340 microplate reader installed with GENESIS-LITE windows based
microplate software.
D. Human tumor
cell lines
NCI-H82
(small cell lung carcinoma), COLO2O5 (colorectal adenocarcinoma), PC-3
(prostate adenocarcinoma), H9 (lymphoma), C32TG (amelanotic melanoma), BT-20
(breast adenocarcinoma), MCF7 (estrogen receptor-positive breast
adenocarcinoma), and H69(AR) (adriamicin-resistant small cell lung carcinoma)
cell lines were obtained from the American Type
Culture Collection (Rockville, MD). NCI-H82, COLO2O5, PC3, H9, and H69(AR)
cells were grown at 37oC in the RPMI 1640 medium with
2mM L-glutamine adjusted to contain 1.5 g/L sodium bicarbonate, 4.5 g/l
glucose, 10 mM HEPES, 1.0 mM sodium pyruvate, and 10% fetal bovine serum.
C32TG, BT-20, and MCF7 cells were propagated at 37oC using the minimum essential medium (Eagle) with 2 mM L-glutamine
and Earl's BSS adjusted to contain 1.5 g/L sodium bicarbonate, 0.1 mM
non-essential amino acids, 1.0 mM sodium pyruvate, and 10% fetal bovine serum.
E.
FACS analysis of surface binding of mAb 2C5 to human tumor cell lines (Iakoubov
and Torchilin, 1997)
Approximately
10,000 cells of different cell lines in each sample were used to check for mAb
2C5 binding using the isotype-matching non-specific UPC10 antibody as a negative
control. Cells were washed with HankÕs balanced salt solution (HBSS) and then
with 1% BSA in PBS, pH 7.4, to prevent a non-specific binding. Cells were then
incubated for 30 min at room temperature with mAb 2C5 or UPC10 and then stained
with fluorescein-conjugated goat anti-mouse IgG. Finally, the cells were fixed
with 4% paraformaldehyde solution in PBS, live-gated using forward vs. side
scatter to exclude debris and dead cells, and analyzed for surface fluorescence
using FACScan (Beckton Dickinson, Franklin Lakes, NJ).
F. Tumors in nude
mice
All
experiments were performed in 6-8 week old female nu/nu mice (Charles River
Laboratories, Wilmington, MA) following protocol #011022 approved by the
Institutional Animal Care and Use Committee in accordance with Principles of
Laboratory Animal Care (NIH publication #85-23, revised in 1985). The animals
were allowed free access to food and water. Approximately 8x106 of
H69(AR) cells, 10-12x106 of COLO2O5, PC3, C32TG, and NCI-H82
cells, or 40x106 of
BT-20 cells in 0.25 ml of RPMI, were inoculated s.c. into the left flanks of
the mice. Mice were examined every 2-3 days until palpable tumors were
detected.
G.
Tumor accumulation of mAb 2C5
Mice with
tumors 1-2 cm in diameter were injected via the tail vein with 111In-labeled
mAb 2C5. After 48 hrs, the mice were anaesthetized and body distribution and
tumor accumulation of mAb 2C5-associated 111In radioactivity was
visualized using an Ohio Nuclear 400 gcamera equipped
with high-energy collimator and Technicare 560 dedicated computer with whole
body pictures taken by digital camera. Tumor and adjacent normal tissues were
then collected, and 111In radioactivity was quantified (as counts
per minute, CPM) using a Beckman 5500B gcounter (Fullerton, CA). Then tumor-to-normal tissue ratios of the
%-injected dose/g of tissue were calculated.
H.
Immunotherapy with mAb 2C5
Immunotherapy was performed
in nude mice with COLO2O5, PC3, NCI-H82, and H69(AR) tumors. Since our previous and current preliminary
experiments have revealed no anti-tumor activity of control injections of PBS
and isotype-matched antibody UPC10, in our full scale experiments, in order to
minimize the number of animals, we have alternatively used as controls PBS or
isotype-matched UPC10 antibody, but normally not both within the same model.
In the model of prophylactic
treatment, nude mice were injected with mAb 2C5 and control PBS, pH 7.4 (in PC3
and NCI-H82 tumor models) or isotype-matched antibody UPC-10 (in COLO2O5 tumor
model) prior to and after the inoculation with tumor cells. 150 mg of mAb 2C5 in 100 ml of PBS or the same
volume/quantity of control injections per mouse were given via tail vein on
days –1, 6, 13 and 19 in COLO2O5- and NCI-H82-bearing mice, and on days
–1, 6 and 13 in PC3-bearing mice. In the established tumor treatment
model, mAb 2C5 and control injections were initiated after the formation of a
visible tumor 7-14 days after the inoculation of tumor cells. Tumor-bearing
mice were injected with mAb 2C5 and control PBS [in PC3, NCI-H82, and H69(AR)
tumor models] or UPC-10 (in COLO2O5 tumor model). 150 mg of mAb 2C5 in 100 ml of PBS or the same
volume/quantity of control injections per mouse were given via tail vein on
days 13 and 20 post inoculation in COLO2O5-bearing mice. In case of PC3-, NCI-H82-,
and H69(AR)-bearing mice, injections were given on days 7, 11 & 15; 7, 14
& 21; and 9, 14, 20, and 27, respectively.
Anticancer
activity of mAb 2C5 was assessed by following the tumor volumes during the
treatment and average tumor weights at the completion of treatment in the
control and mAb 2C5-treated groups. The apparent tumor volume was calculated on
different days during the treatment using the formula (Geran et al, 1972),
tumor volume (mm3) = (Length X Width2)/2, length being
greater than width. At the end of treatment, the mice were sacrificed and
tumors were removed and weighed.
I.
Statistics
Differences
in apparent tumor volumes during the treatment and post-mortem tumor weights
were compared using the non-parametric two-tailed Wilcoxon rank sum test for
two independent samples. For easy representation of the difference in tumor
volumes during the treatment, the average tumor volume (mm3) of the
group vs. days after tumor cell inoculation was plotted. Tumor weights were
plotted as box plots that represent the group median, quartiles and extremes.
III. Results
A. Properties of mAb 2C5
We confirmed the purity of mAb 2C5 by the presence of
the single peak in the protein G column antibody elution profile and the single
band corresponding to an IgG protein after polyacrylamide gel electrophoresis (Figure 1, A,B). We have also confirmed
antibody immunoreactivity against NSs purified from the rat liver (Li et al,
1995) using a standard ELISA protocol (Figure
1, C).
The determination of mAb 2C5 KD with monoNS
is presented on Figure 2 (here, the
KD value characterizes avidity or relative affinity because of
bivalent nature of an antibody).
autoimmunity
was seriously considered as an antineoplastic therapeutic strategy (Pardoll,
1999). Though the exact autoimmune components with antitumor function are not
known, ANAs seem to be a good candidate.
Two major mechanisms of action are presently being
considered to explain anti-tumor activity of therapeutic monoclonal antibodies
(Houghton and Scheinberg, 2000). The first is based on the antibody-mediated
killing of tumor cells by various immune effectors such as complement or
cytotoxic immune cells. The second involves antibody bioactivity un-related to
immunologic function, such as blocking the access of growth factors to tumor
cells or tumor vasculature. A convincing case for the in vivo involvement of immune effectors in monoclonal
antibody-based tumor suppression was obtained recently in immunocompetent as
well as athymic mice (Clynes et al, 2000). However, for each particular
antibody, the conclusion on the involvement of immune killing is traditionally
based on the indirect evidence, where the ability of the antibody to mediate
complement- or cytotoxic cell-dependent killing is demonstrated in vitro (Herlyn et al 1980). In
addition, according to this in vitro
criteria, effector cells from nude mice are known to mediate levels of ADCC of
equal or even greater magnitude than cells from normal mice (Kohl et al, 1984).
Our in vitro data on the ability of
mAb 2C5 to mediate ADCC serve as indirect evidence for this mechanism of tumor
suppression in both syngeneic tumor models in normal mice (Iakoubov and
Torchilin, 1997) and xenogeneic models in nude mice.
We can also reasonably expect at least one additional
activity for the mAb 2C5. Since most tumors are expected to bear NSs on the
surfaces of apoptotic cells (Radic et al, 2004) and result in elevated blood
NSs (Holdenrieder et al, 2001), external anti-NS antibodies should lead to
elevated immune complexes known to activate the immune system (Lucisano,
Mantovani, 1984). This activation could be of a significant importance in
opposing the tumor-mediated immunosuppression characteristic of cancer patients
(Pollock, Roth, 1989). Thus, the efficiency of mAb 2C5 and similar antibodies
might be in part based on their ability to turn on some additional immune
mechanisms not characteristic for conventional immunization-induced monoclonal
antibodies. In addition to their probable ability to block to a certain extent
the earlier mentioned NK-inhibiting action of extracellular NSs (chromatin) (Le
Lann-Terisse et al, 1994, 1997), these antibodies can also interfere with the
recently reported neoangiogenic activity of NSs (Tanner, 2003). The competition
between NS-specific antibodies and C-reactive protein (Robey et al, 1985) for
the binding with chromatin may exist in the blood, however the results of our
experiments clearly demonstrate that in
vivo the activity of mAb 2C5 is not blocked by this hypothetical
competition.
Earlier, monoclonal antibodies belonging to IgG2a and
IgG3 isotypes have been described demonstrating ADCC against tumor cells
over-expressing corresponding antigens, such as anti-ganglioside antibodies
(Lin et al, 2001; Nakamura et al, 2001; Parajuli et al, 2001). However, these
antibodies have been obtained by immunization and, to the best of our
knowledge, none of them was ever shown to demonstrate anti-tumor activity
against a variety of unrelated human tumors.
As potential anti-tumor agents, natural ANAs may have
a number of advantages compared to conventional anti-tumor antibodies. ANAs
appear to be effective against a broad spectrum of various tumor types. Their
anti-tumor mechanisms are probably multimodal and hence more efficient. Their
side-effects should be minimal, since their natural presence in the blood does
not seem to be harmful to the host. In addition, assuming that the ADCC and
other immune effectors possibly activated by circulating mAb 2C5/NS
immunocomplexes are independent of MDR mechanisms, such as the p-glycoprotein
pump, mAb 2C5 and similar antibodies might serve as a treatment of choice
against MDR tumors. This assumption is well supported by our results with the
H69(AR) tumor. One can also speculate that such antibodies may be used together
with apoptosis-inducing agents required to convert the tumor cell chromatin
into NSs and subsequently provoke the release of these NSs and their binding to
the surface of living tumor cells to make them better targets for the
antibodies.
The question if the mAb 2C5
(and similar antibodies) only inhibit tumor growth and have to be used as a
component of the combination therapy, or, if optimized administration protocols
are established, they can completely eliminate tumors, as well as the exact
nature of NS-binding sites on the surface of tumor cells and major mechanisms
of anti-tumor activity of NS-restricted ANAs are currently under investigation
in our laboratory.
Acknowledgements
This study was funded in part by the NIH grant R01
EB02995 to VPT. The authors would like also to acknowledge the
researcher-friendly policy of partial overhead return at Northeastern
University.
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