PMCID:
PMC2687140
PMID:
19049251
Unexpected Antitumorigenic Effect of Fenbendazole when
Combined with Supplementary Vitamins
Abstract
Diet containing the anthelminthic fenbendazole is used
often to treat rodent
pinworm infections because it is easy to use and has few
reported adverse effects on research. However, during fenbendazole treatment at
our institution, an established human lymphoma xenograft model in
C.B-17/Icr-prkdcscid/Crl
(SCID) mice failed to grow. Further investigation revealed that the
fenbendazole had been incorporated into a sterilizable diet supplemented with
additional vitamins to compensate for loss during autoclaving, but the diet had
not been autoclaved. To assess the role of fenbendazole and supplementary
vitamins on tumor suppression, 20 vendor-supplied 4-wk-old SCID mice were
assigned to 4 treatment groups: standard diet, diet plus fenbendazole, diet
plus vitamins, and diet plus both vitamins and fenbendazole. Diet treatment was
initiated 2 wk before subcutaneous flank implantation with 3 × 107
lymphoma cells. Tumor size was measured by caliper at 4-d intervals until the
largest tumors reached a calculated volume of 1500 mm3. Neither diet
supplemented with vitamins alone nor fenbendazole alone caused altered tumor
growth as compared with that of controls. However, the group supplemented with
both vitamins and fenbendazole exhibited significant inhibition of tumor
growth. The mechanism for this synergy is unknown and deserves further
investigation. Fenbendazole should be used with caution during tumor studies
because it may interact with other treatments and confound research results.
Abbreviation: HIF,
hypoxia-inducible factor 1α
Pinworms
are a common problem in rodent facilities4,16and
typically are treated with anthelminthics.17
Fenbendazole incorporated in the diet is used often because it is safe—the oral
LD50 for rats and mice is in excess of 10,000 mg/kg5—and
labor-efficient, and adverse effects in research rodents have rarely been
reported.20
More than 50% of ingested fenbendazole is absorbed and metabolized in the
liver, primarily to the active form, fenbendazole sulfoxide.19
Fenbendazole inhibits microtubule polymerization, and its efficacy as an
anthelminthic results from its greater affinity for helminth tubulin than
mammalian tubulin.9
During
an 8-wk facility treatment for Aspiculuris tetraptera pinworms with
fenbendazole diet at our institution, human lymphoma xenografts failed to grow
in C.B-17/Icr-Prkdcscid/Crl (SCID) mice. This
well-established xenograft model is used to study the role of mitochondrial
genes in tumorigenesis and usually results in 80% to 100% successful tumor
growth within 21 d. However, during the facility treatment with fenbendazole,
no tumors grew in 40 mice during the 30 d after injection. The mice in this
study had not been diagnosed with pinworms but were part of a facility
treatment. Rodents in this area customarily were fed a commercial irradiated
diet (Global 2918, Harlan Teklad, Madison, WI). However the equivalent
treatment diet containing 150 ppm fenbendazole was available only in a
sterilizable form (2018S, Harlan Teklad) supplemented with vitamins A, D, E, K,
and B (Table 1) to compensate for loss during sterilization. Because the animal
facility was not configured for dietary sterilization, the sterilizable diet
was fed unautoclaved, with the result that mice received higher-than-normal
concentrations of vitamins. Therefore the observed antitumor effect could have
resulted from either the additional vitamins or the fenbendazole. Therefore a
controlled study was conducted to test whether fenbendazole, supplemented
vitamins, or both in combination affected the growth of this human lymphoma
cell line in SCID mice.
Materials
and Methods
Mice
were housed in an AAALAC-accredited facility under conditions compliant with
the Guide for the Care and Use of Laboratory Animals.12
Procedures were approved by the Johns Hopkins institutional animal care and use
committee. The mice were housed in individually ventilated cages (Allentown
Caging Equipment, Allentown, NJ) on autoclaved corncob bedding (Bed-O'Cobs, The
Andersons, Maumee, OH). Mice received hyperchlorinated reverse-osmosis–treated
water by means of an in-cage automated watering system (Edstrom Industries,
Waterford, WI). Cages were changed by using chlorine-dioxide-based disinfectant
(MB10 tabs, 100-ppm solution, Quip Laboratories, Wilmington, DE) in
filtered-air change stations (Lab Products, Seaford, DE). The colony tested
free of a wide range of viral and parasitic pathogens by sentinel surveillance;
pathogens included Sendai virus, pneumonia virus of mice, mouse hepatitis
virus, mouse minute virus, mouse parvovirus 1 and 2, Theiler mouse
encephalomyelitis virus, reovirus, epizootic diarrhea of infant mice,
lymphocytic choriomeningitis virus, ectromelia virus, murine adenovirus, murine
cytomegalovirus, Mycoplasma pulmonis, fur mites, and pinworms.
Twenty
4-wk-old male SCID mice (Charles River Laboratories, Boston, MA) were assigned
randomly to 4 groups housed 5 animals per cage: control diet (2018, Harlan
Teklad), diet plus fenbendazole (2018 custom-formulated with 150 ppm
fenbendazole, Harlan Teklad), diet plus supplemented vitamins (2018S, Harlan
Teklad), and diet plus both fenbendazole and supplemented vitamins (2018S plus
150 ppm fenbendazole, Harlan Teklad). All diets had the same basic composition
(18% protein, 5% fat; Table 1), and none of the diets was autoclaved. The mice
were stabilized on their respective diets for 2 wk after arrival and before
tumor cells were injected.
Table
1.
Vitamin
levels in nonsterilizable (regular) and sterilizable (supplemented) diets
|
Diet
|
||||
|
Vitamins
|
Regular
|
Supplemented
|
Units
|
% Increase
|
|
A
|
15.4
|
30.7
|
IU/g
|
100
|
|
Retinol
|
4.65
|
9.31
|
mg/kg
|
100
|
|
D3
|
1.54
|
2.05
|
IU/g
|
33
|
|
Cholecalciferol
|
38.39
|
51.18
|
g/kg
|
33
|
|
E
|
101
|
126
|
mg/kg
|
25
|
|
K3
|
51
|
102
|
mg/kg
|
100
|
|
B1
|
16.5
|
117.6
|
mg/kg
|
613
|
|
B2
|
14.9
|
27.2
|
mg/kg
|
83
|
|
Available
niacin
|
41.2
|
87.3
|
mg/kg
|
112
|
|
B6
|
18.5
|
26.8
|
mg/kg
|
45
|
|
Pantothenic
acid
|
33
|
141.6
|
mg/kg
|
329
|
|
B12
|
0.08
|
0.15
|
mg/kg
|
88
|
|
Available
biotin
|
0.3
|
0.82
|
mg/kg
|
173
|
|
Folate
|
3.34
|
8.41
|
mg/kg
|
152
|
The
data shown are vendor-reported values.
The
day after arrival, blood was collected by puncture of the facial vein under
manual restraint and processed by using an automated analyzer (Hemavet 950,
Drew Scientific Group, Dallas, TX) for complete blood count. Human Burkitt
lymphoma cells (P493-6 B cell line8) were cultured in RPM1 1640 plus
10% fetal calf serum containing 100 U/ml penicillin and 100 µg/ml streptomycin.
The cells were washed, counted, and resuspended in PBS. Each mouse was
restrained manually and received 3 × 107 lymphoma cells in 100 µL
PBS injected subcutaneously in the flank. Growth of tumors was monitored every
4 d by using calipers, and tumor volume was calculated by using the formula
length × width × width × 0.52 mm3. Once the largest tumors reached a
calculated volume of 1500 mm3, the experiment was terminated. Before
euthanasia of mice, blood was collected from the facial vein and analyzed for
complete blood count. The size of tumors in each group at the endpoint was
compared with that of the control group by using the Student t test.
Total white cell, lymphocyte, and neutrophil counts were compared with those of
controls at the beginning and end of the experiment.
Results
Tumor
size.
Tumors
in the fenbendazole plus vitamin group were significantly smaller (P =
0.009) and delayed in initial growth compared with those of the control group (Figure 1). Tumor growth did not differ
between control and fenbendazole-only (P = 0.12) or vitamin-only (P
= 0.82) groups. The apparent trend toward increased tumor size (P =
0.12) in the fenbendazole-only group was due to a single outlier.
Growth
in tumor volume (mean ( SD) in mice on 4 different diets. After subcutaneous
injection of lymphoma cells, tumor growth in mice receiving fenbendazole- or
vitamin- supplemental diet did differ from that in controls. Tumor growth in
mice on fenbendazole- plus vitamin-supplemented diet was significantly (P =
0.009) inhibited compared with that in controls.
White
cell counts.
One
mouse died during the initial blood collection, and 1 blood sample from the
terminal group was lost. Initial complete blood counts (Figure 2) were typical of SCID mice,
demonstrating a low white cell count with a paucity of lymphocytes. White cell
counts did not differ significantly between test and control groups on arrival.
At the end of the study (Figure 2), all groups demonstrated a
leukocyte response consisting primarily of neutrophils. The total white cell
and neutrophil responses in the fenbendazole plus vitamin group were
significantly smaller (P = 0.001 and P = 0.04, respectively) than
in the control group. There was a trend (P = 0.06) toward increased
total white cell count and a significantly increased lymphocyte count (P
= 0.009) in the fenbendazole-only group compared with controls.
Initial
and terminal white cell counts (mean ± SD) in mice on 4 different diet. Initial
counts did not differ among the 4 groups. Terminal total white cell and
neutrophil counts in mice receiving the (p=0.001 and p=0.04 respectively) lower
than those in control animals, and terminal lymphocyte counts in the
fenbendazole-only group were significantly (P = 0.009) higher than those in
controls.
Discussion
This
study demonstrated that a combination of supplemented vitamins and fenbendazole
in the diet inhibited growth of a human lymphoma cell line in SCID mice,
whereas fenbendazole or vitamins alone had no growth inhibitory effect. The
mechanism for this synergy is as yet unknown. However, like other anticancer
drugs such as taxanes,14
quinolones,3
and vinca alkaloids,15
fenbendazole inhibits microtubule polymerization. In addition, fenbendazole is
a member of a large group of related anthelminthics, the benzimidazoles, and
another member of this group, mebendazole, exerts antitumor effects by
inhibition of tumor-induced neovascularization.11
However, in the present case, fenbendazole likely contributes to the
antitumorigenic effect through its antimicrotubule activity.
Supplemented
vitamins included B, D, K, E, and A. Vitamins E and A both have antitumor
properties by virtue of their antioxidant properties. Vitamin E causes
antitumor and antimetastatic effects in several animal models of cancer; for
example, it suppresses the nuclear transcription factor NFκB in prostate cell
lines.13
NFκB regulates proapoptotic and prometastatic proteins; thus suppression
results in antitumor effects. Higher intake of dietary folate and vitamin B has
been associated with lower incidence of colorectal cancer in women.22
Recent work suggests that hypoxia-inducible factor 1α (HIF), which plays a key
role in tumorigenesis by facilitating adaptation to hypoxia, is diminished by
microtubule inhibitors,7
and some antioxidants may exert their antitumor effects through reducing HIF rather
than by reducing genetic instability.8,10
We hypothesize that the combination of fenbendazole and supplemented vitamin
antioxidants may have exerted a threshold effect, resulting in reduction of HIF
and inhibition of tumorigenesis. Indeed, preliminary information from our
laboratory confirms that fenbendazole inhibits HIF transcriptional activity in
cell culture in an additive manner with other HIF inhibitors (data not shown).
This
study demonstrated significant inhibition of tumor growth. Results were less
dramatic than the total inhibition initially observed, perhaps due to
inadvertent inclusion of lower vitamin concentrations during the study than
during the initial observation. Vitamins in prepared diets deteriorate with
time, and the study diet containing both vitamins and fenbendazole was within a
week of its expiration date (6 mo after manufacture) at the time of this study.
In contrast, diet used during the initial observation was newly ordered to
treat the pinworm outbreak and so was likely more recently manufactured, with
higher vitamin concentrations. Unfortunately expiration dates during the
initial observation were not recorded and vitamin concentrations in the diet
were not analyzed independently so this theory cannot be confirmed.
Figure 1 shows a trend (P = 0.12)
toward increased tumor growth in the fenbendazole only treatment group.
This trend was the result of 1 outlier. Nonetheless, fenbendazole may have
tumor-promoting activity in rats at therapeutic dosages (that is, through
inhibition of connexin 32 and induction of cytochrome P450 enzymes 1A1 and
1A2).21
In our experiment, the apparent increase in tumor size in the fenbendazole
group was due to a single large-tumor outlier, and we believe that this trend
is due to experimental noise. Further studies are needed to determine whether
fenbendazole actually exhibits a tumor-promoting effect in this model.
Although
the exact composition of T and B cells was not analyzed, complete blood counts
confirmed that the numbers of white cells did not differ initially between the
treatment and control groups, ruling out the possibility of a chance
concentration of relatively immunocompetent ‘leaky’ SCID mice1,2
in 1 group. At study termination, the fenbendazole plus vitamin group had
significantly lower total white cell and neutrophil values (P = 0.001
and P = 0.04, respectively) than did the control group. This observation
is consistent with significantly smaller tumors causing less compression and
necrosis of adjacent tissues, although this supposition was not confirmed by
histopathology. There was also a trend (P = 0.06) toward increased total
numbers of white cells and a significantly larger (P = 0.009) lymphocyte
response in the fenbendazole-only group. Fenbendazole has had immunomodulatory
effects in sheep and mice18
and stimulated proliferation of T and B cells in healthy mice,6
but most studies have shown no effect on selected immune responses.21
It is not possible to draw any conclusions regarding immunomodulation from the
present study because additional analysis of cell types was not done.
Our
study showed that fenbendazole alone did not significantly affect growth of the
P493-6 human lymphoma cell line in SCID mice. Most importantly, our observation
that fenbendazole in combination with supplemented vitamins significantly inhibited
tumor growth has implications for its use during antitumor studies because it
may cause unpredictable interactions with test substances and thus alter
research results.
Acknowledgments
This
study was in part supported by Leukemia Lymphoma Society grant LLS6175-08, NIH
grant CA57341, and by Johns Hopkins Research Animal Resources.
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