From the Departments of Medicine and of Biochemistry and Molecular Pharmacology, Jefferson Medical College, Philadelphia, Pennsylvania 19107
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ABSTRACT |
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T-84 and Caco-2 human colon carcinoma cells and Madin-Darby canine kidney (MDCK) cells were used to study binding and transcytosis of iodinated Clostridium botulinum neurotoxin serotypes A, B, and C, as well as tetanus toxin. Specific binding and transcytosis were demonstrated for serotypes A and B in intestinal cells. Using serotype A as an example, the rate of transcytosis by T-84 cells was determined in both apical to basolateral (11.34 fmol/h/cm2) as well as basolateral to apical (8.98 fmol/h/cm2) directions, and by Caco-2 cells in the apical to basolateral (8.42 fmol/h/cm2) direction. Serotype A retained intact di-chain structure during transit through T-84 or Caco-2 cells, and when released on the basolateral side was toxic in vivo to mice and in vitro on mouse phrenic nerve-hemidiaphragm preparations. Serotype C and tetanus toxin did not bind effectively to T-84 cells, nor were they efficiently transcytosed (8-10% of serotype A). MDCK cells did not bind or efficiently transcytose (0.32 fmol/h/cm2) botulinum toxin. Further characterization demonstrated that the rate of transcytosis for serotype A in T-84 cells was increased 66% when vesicle sorting was disrupted by 5 µM brefeldin A, decreased 42% when microtubules were disrupted by 10 µM nocodazole, and decreased 74% at 18 °C. Drugs that antagonize toxin action at the nerve terminal, such as bafilomycin A1 (which prevents acidification of endosomes) and methylamine HCl (which neutralizes acidification of endosomes), produced only a modest inhibitory effect on the rate of transcytosis (17-22%). These results may provide an explanation for the mechanism by which botulinum toxin escapes the human gastrointestinal tract, and they may also explain why specific serotypes cause human disease and others do not.
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INTRODUCTION |
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Botulinum neurotoxin (BoNT),1 which is the etiologic agent responsible for the disease botulism, can enter the body by several different routes, but the most common of these is the gastrointestinal system (1-4). Thus, most cases of intoxication are due to ingestion of food contaminated with preformed toxin or ingestion of food contaminated with bacteria that can produce toxin in the gut. In either case, BoNT escapes the gastrointestinal system to reach the general circulation (lymph and blood). Toxin in the blood is then distributed to peripheral cholinergic nerve endings, which are the target cells for toxin action.
There is now a substantial literature describing the cellular, subcellular, and even molecular aspects of toxin action on cholinergic cells (5-9). This literature derives from a model that envisions the toxin proceeding through three major steps (2, 10-13). During the first step, the toxin binds to receptors that are highly localized in the junctional region of cholinergic cells. The toxin molecule, which is composed of a heavy chain (Mr ~100,000) and a light chain (Mr ~50,000) linked by a disulfide bond, is thought to rely on the carboxyl terminus of the heavy chain to associate with cells. During the second step, the toxin is productively internalized by vulnerable cells. This process is actually a sequence of two events: 1) penetration of the plasma membrane by receptor-mediated endocytosis, and 2) penetration of the endosome membrane by pH-induced translocation. Although there is much that remains to be determined about productive internalization, there is suggestive evidence that the amino terminus of the heavy chain plays an important role in this process. During the third and final step in toxin action, the light chain that reaches the cytosol acts as a zinc-dependent endoprotease to cleave polypeptides that are essential for exocytosis (6, 8, 9). Blockade of exocytosis leads to the failure of neuromuscular transmission that is characteristic of botulism.
In contrast to our knowledge of events at the nerve ending, very little is known about the cellular and subcellular events that account for the ability of the toxin to cross membranes in the gastrointestinal system (14-16). Those data that are available suggest that the mouth is the least effective site of absorption, the stomach is intermediate, and the intestine is the most effective site of absorption. There are no studies that actually demonstrate a mechanism for botulinum toxin penetration of gut cells. However, there is one self-evident matter that can be deduced. The series of steps that underlie toxin movement at the level of individual gut cells cannot be identical to the steps that underlie toxin movement in individual nerve cells. If BoNT were to enter and remain inside cells in the gastrointestinal system, this would prevent it from reaching peripheral cholinergic nerve endings. Thus, there must be fundamental differences that distinguish toxin movement across gastrointestinal membranes and movement across neuronal membranes.
There are two broad categories of toxin transport that could account for movement from the gastrointestinal system to the general circulation. As proposed by Bonventre (16), transport could involve a specific, receptor-mediated mechanism or a nonspecific mechanism. In the present study, work has been done to test the hypothesis that BoNT crosses the gut wall by the process of specific binding and transcytosis. According to this hypothesis, there should be little or no pH-induced translocation of toxin molecules across intracellular membranes. Instead, this hypothesis requires that toxin bound on the lumenal side of cells must be delivered to the serosal side of cells, and furthermore the transcytosed toxin must be in a conformation that can act upon cholinergic nerves. This hypothesis has been tested by studying the binding, movement, and residual toxicity of BoNT type A (BoNT/A) added to a human epithelial cell line of gut origin (T-84). The resulting data provide the first insights into the cellular and subcellular events that account for toxin movement from the gastrointestinal system to the general circulation.
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EXPERIMENTAL PROCEDURES |
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Materials-- T-84 human colon carcinoma cells, Caco-2 human colon carcinoma cells, and Madin-Darby canine kidney cells were obtained from The American Type Culture Collection (Rockville, MD). Tissue culture media and sera were purchased from Life Technologies, Inc. [3H]Inulin and 125I-Bolton-Hunter reagent were purchased from NEN Life Science Products. Reagents were purchased from Sigma, and tissue culture supplies were obtained from Fisher. Sephadex G-25 gel filtration columns were obtained from Amersham Pharmacia Biotech. Tetanus toxin was purchased from Calbiochem (Behring Diagnostics, La Jolla, CA). A sample of BoNT/A-associated proteins was kindly provided by Dr. Bibhuti DasGupta (University of Wisconsin-Madison, Madison, WI). Samples of BoNT/C were kindly provided by Dr. Y. Kamata (University of Osaka Prefecture, Osaka, Japan). BoNT/A and BoNT/B were purified according to procedures described in the literature (17-19).
Animals-- Swiss-Webster mice (female, 20-25 g), which were purchased from Ace Animals (Boyertown, PA), were housed in an American Association for Accreditation of Laboratory Animal Care-accredited animal colony and allowed unrestricted access to food and water. All procedures involving animals were reviewed and approved by the Thomas Jefferson University Institutional Animal Care and Use Committee.
Cell Culture-- T-84 cells were grown in a 1:1 mixture of Dulbecco's modified Eagle's medium (1 g/liter D-glucose) and Ham's F-12 nutrient medium supplemented with 5% newborn calf serum, 100 units/ml penicillin, 100 µg/ml streptomycin, 8 µg/ml ampicillin, and 15 mM Hepes. Cultures were maintained at 37 °C in 6% CO2. T-84 cells were fed every 3 days and passaged (1:2) when 95% confluent, approximately every 6 days. Passages 55 through 76 were used for experiments described in this report.
Caco-2 cells were grown in Dulbecco's modified Eagle's medium (4.5 g/liter D-glucose) supplemented with 15% newborn calf serum, 100 units/ml penicillin, 100 µg/ml streptomycin, and 15 mM Hepes. Cultures were maintained at 37 °C in 6% CO2. Caco-2 cells were fed every 2 days and passaged (1:2 split ratio) when 95% confluent, approximately every 6 days. Passages 20 through 29 were used for experiments described in this report. MDCK cells were grown in Dulbecco's modified Eagle's medium (4.5 g/liter D-glucose) supplemented with 10% newborn calf serum, 100 units/ml penicillin, 100 µg/ml streptomycin, and 25 mM Hepes. Cultures were maintained at 37 °C in 6% CO2. MDCK cells were fed every 3 days and passaged (1:5) when 95% confluent, approximately every 3 days. Passages 56 through 75 were used for experiments described in this report.Inulin Flux-- To control for membrane integrity and to estimate diffusion between cells, the rate of passage of [3H]inulin from the upper to the lower reservoir was determined essentially as described previously (20). According to this procedure, the medium in both reservoirs contained unlabeled 1 mM inulin. The assay was initiated by addition of [3H]inulin to the upper reservoir. Rates for inulin flux from the upper to the lower wells were determined for 2, 6, or 20 h.
To control for nonspecific effects that might be caused by prolonged incubation of cells with toxin, inulin flux experiments were repeated on cultures that had been preincubated with 1 × 10Iodination--
BoNT/A, B, and C, and tetanus toxin, as well as
toxin-associated proteins such as the hemagglutinins, were iodinated
using 125I-Bolton-Hunter reagent (NEN Life Science
Products) essentially according to manufacturer's instructions. The
reaction time was reduced in order to diminish the loss of toxicity of
the resulting product. The toxins were labeled to an average specific
activity of 500 Ci/mmol with a residual toxicity of greater than 90%
(21-23). Pure neurotoxin (250 µg) in borate buffer (pH 7.8, 200 µl) was added to dried, iodinated ester and reacted on ice for 15 min. The reaction was terminated by addition of 50 µl of 1 M glycine in borate buffer for 5 min. The total reaction
mixture (250 µl) and rinse (250 µl) were loaded onto a Sepahadex
G-25 column that was preequilibrated with filtration buffer (150 mM Na2HPO4, 150 mM
NaCl, 0.1% gelatin, pH 7.4). The labeled toxin was eluted with filtration buffer, and 0.5-ml fractions were collected. An aliquot (5 µl) of each fraction was assayed for radioactivity. The labeled toxin
peak, which eluted at void volume, was pooled and stored at 3 °C.
Toxin concentration in the pooled fraction was determined spectrophotometrically at 278 nm using the following relationship, 1.63 A278 = 1 mg/ml (18). A portion of this sample
was counted in a -counter to ascertain the number of counts
(disintegrations/min) present. Sample concentration and associated
counts were used to calculate specific activity.
Toxin Binding Assay--
Cells were grown, differentiated, and
induced to polarize as described above. Cells were rinsed three times
and then incubated in mammalian Ringers solution with 10 mM
HEPES and 1 mg/ml bovine serum albumin, pH 7.4. The cells were slowly
(~2 h) cooled to 3 °C. The buffer in the upper well was replaced
with cold buffer (3 °C) containing 125I-BoNT, with or
without a 50-fold molar excess of unlabeled toxin. The cells were
incubated at 3 °C for 3 h to allow sufficient time to reach
equilibrium, after which cells and membranes were washed 3 times with
Hanks' balanced salt soluiton plus 10 mM HEPES with 1 mg/ml bovine serum albumin. Membranes were then cut out of the Transwell® holders and placed in a -counter. At least three
replicates per condition were included.
Transcytosis Assay-- For assay of botulinum neurotoxin transcytosis, cells were grown in Transwell® porous bottom dishes on polycarbonate membranes with a 0.4 µm pore size. The growth area within each insert was 1 cm2. Prior to being seeded with cells, the Transwells were coated with 10 µg/cm2 rat tail collagen type I. Briefly, rat tail collagen stock solution (6.7 mg/ml) was prepared in sterile 1% acetic acid and stored at 3 °C. The stock solution was diluted in acidified 60% ethyl alcohol, as needed, and 150 µl containing 10 µg of diluted collagen were added to each well. The coated wells were allowed to dry at room temperature overnight (18 h). After drying, the wells were sterilized under UV light for 1 h, followed by a preincubation with cell culture medium (30 min). The preincubation medium was removed immediately prior to addition of cells and fresh medium.
Cells (T-84, Caco-2 or MDCK) were plated at confluent density (~1.5 × 105 cells) into the Transwells with 0.5 ml of medium in the upper chamber and 1.0 ml in the lower chamber. In these experiments, medium in the upper chamber bathed the apical (or mucosal) surface of cells, and medium in the lower chamber bathed the basolateral (or serosal) surface of cells. Culture medium was changed every 2 days. The cultures were allowed to differentiate for a minimum of 10 days before assay of transcytosis. The formation of tight junctions was experimentally confirmed by measuring the rate of [3H]inulin movement from the upper chamber into the lower chamber (see above). Experiments were performed on cultures that were between 10 and 15 days old. The transcytosis assay was initiated by adding 1 × 10Cell Fractionation--
Cell fractions for assay of
intracellular toxin were prepared by standard methods. Briefly, BoNT/A
(1 × 108 M) was added to the upper
reservoir at 37 °C for 1 h. The wells were subsequently cooled
to 18 °C over a 45-min time period, after which the cells were
washed five times (upper and lower surface) with cold Dulbecco's
phosphate-buffered saline without Ca2+ or Mg2+.
Cells were trypsinized at 37 °C for 10 min, washed once with medium,
then twice with homogenization buffer (255 mM sucrose, 1 mM EDTA, 20 mM Hepes, pH 7.4) containing
protease inhibitors (5 µM antipain, 1 µM
aprotinin, 10 µM leupeptin, 5 µM pepstatin A, 100 µM phenylmethylsulfonyl fluoride). Harvested cells
were homogenized at 3 °C (on ice) in a glass-Teflon homogenizer
(2 × 20 strokes). The homogenate was fractionated using an SS-34 rotor in a Sorvall RC5B centrifuge (Sorvall, Inc., Newtown, CT.). Homogenates were spun at 1000 × g for 5 min. The
resulting supernatant (S-1) was recentrifuged at 10,000 × g for 10 min. The second supernatant (S-2) was used for
determination of cytosolic toxin.
Electrophoresis-- Samples for autoradiographic analysis were separated on 7.5% polyacrylamide gels according to Laemmli (24), using reducing or non-reducing conditions. Gels were fixed for 30 min in destaining buffer, dried on blotter paper, and exposed to film (HyperfilmTM MP, Amersham Pharmacia Biotech).
In Vivo and in Vitro Toxicity Testing-- The toxicity of transcytosed BoNT/A that was collected from the lower reservoir was bioassayed either by intraperitoneal injection into mice or by addition to mouse phrenic nerve-hemidiaphragm preparations. For the in vivo bioassay, transcytosed toxin or native toxin was administered in a 100-µl aliquot of Dulbecco's phosphate-buffered saline with 1 mg/ml bovine serum albumin, per animal. Animals were checked for survival over the 12-h duration of the experiment.
For the in vitro bioassay, tissues were excised and suspended in physiological buffer that was aerated with 95% O2, 5% CO2 and maintained at 35 °C. The physiological solution had the following composition (millimolar): NaCl, 137; KCl, 5; CaCl2, 1.8; MgSO4, 1.0; NaHCO3, 24; NaH2PO4, 1.0; D-glucose, 11; and gelatin, 0.01%. Phrenic nerves were stimulated continuously (1.0 Hz; 0.1-0.3-ms duration), and muscle twitch was recorded. Toxin-induced paralysis was measured as a 50% reduction in muscle twitch response to neurogenic stimulation. For both in vivo and in vitro bioassays, it was necessary to quantify the amount of toxin that was recovered and tested. This was done in two ways. First, the aliquot to be tested was submitted to gel filtration chromatography to isolate the toxin peak. The specific activity of the starting material added to the upper chamber of the Transwell® apparatus was calculated immediately after iodination (see "Iodination"). The number of counts in the purified fraction from the aliquot taken from the lower chamber and the specific activity were used to calculate the amount of toxin. Second, the actual rates of transcytosis as determined in this study (e.g. Table I) were used to calculate the amount of the toxin in the aliquots that were tested.Statistical Analyses-- All data derived from three or more separate experiments are presented as means ± S.E. The equality of variances was tested using the F test. Subsequently p values were calculated using either a two-sample t test for independent samples with equal variances or a two-sample t test for independent samples with unequal variances (Cochran's method).
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RESULTS |
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Inulin Flux-- Experiments were done both to confirm the formation of tight junctions in cell cultures and to assess the rate of movement of molecules across these tight junctions. For this purpose, [3H]inulin flux was measured over periods of 2-20 h. The average values obtained in three experiments indicated that the rate of [3H]inulin flux from the apical to the serosal side of T-84 cells typically fell within the range of 0.01- 0.07 nmol/h/cm2. The rates were slightly lower for Caco-2 and MDCK cultures. These rates compare favorably with those reported by others (20), and they are a strong indication that tight junctions had been formed and molecular diffusion was hindered.
Identical experiments were done on cultures that had been pretreated with 1 × 10125I-Labeled Toxin Binding-- Several serotypes of botulinum toxin and tetanus toxin were iodinated, and the ability of these ligands to bind to intact cells was measured. As shown in Fig. 1, there was substantial and nearly equivalent binding of serotypes A (19.44 ± 2.35 fmol/cm2) and B (18.33 fmol/cm2) to T-84 cells. In contrast, the binding of serotype C (0.22 fmol/cm2) and tetanus toxin (0.47 fmol/cm2) was negligible.
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Transcytosis of Clostridial Toxins-- Experiments were done to test the ability of differentiated, polarized T-84 epithelial cells to transcytose botulinum neurotoxin types A, B, and C, as well as tetanus toxin. Similar experiments were done on MDCK cells, which have the ability to differentiate, polarize, and transcytose, but which have not been implicated in clostridial toxin action. Fig. 2, which illustrates data obtained for iodinated, homogeneous serotype A, clearly shows that T-84 cells are capable of uptake, transcytosis, and release of toxin. In contrast, MDCK cells did not transcytose serotype A at a significant rate.
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Effects of Concentration on the Rate of BoNT/A
Transcytosis--
Data presented thus far indicate that T-84 cells
transcytose BoNT/A. The experiments illustrated in Fig.
3 show that increases in toxin
concentration were associated with increases in transcytosis in T-84
cells. The rates of apical basolateral transcytosis increased
600-fold from 0.262 fmol/cm2/h at 10
10
M to 168.50 fmol/cm2/h at 10
7
M toxin. Conversely, the fractional amount of toxin added
to the top well (Fig. 3, numbers in parentheses) that was transported across cells decreased 2-fold from 12% at 10
10
M to 6% at 10
7 M in T-84
cultures. When equivalent experiments were done on MDCK cells, there
was much less indication of a dose-dependent capacity for
transcytosis.
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Further Characterization of BoNT/A Transcytosis--
Data
presented thus far demonstrate that polarized human epithelial cells
transcytose certain clostridial toxins. Therefore, serotype A was
selected as a prototype, and further work was done to establish rate
constants. In addition, an effort was made to compare apical basolateral transcytosis with basolateral
apical transcytosis. The
data on rate constants are presented in Table I.
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Effects of Brefeldin A, Nocodazole, and Temperature on Transcytosis of BoNT/A-- Several drugs and procedures were used to further characterize the process of toxin movement across cells. Each drug and procedure was selected on the basis that previous studies have shown them to increase or decrease transcytosis (25-29).
Fig. 4 summarizes the results of the studies with brefeldin A, which has been shown to disrupt vesicle sorting; nocodazole, which has been shown to disrupt microtubules; and temperature. Transcytosis of BoNT/A was significantly increased (p < 0.01) by incubation of cells with 5 µM brefeldin A, whereas the rate of transcytosis was significantly decreased (p < 0.001) by incubation with 10 µM nocodazole. In keeping with expectations, transcytosis of the toxin was significantly decreased (p < 0.001; ~75%) when temperature was lowered from 37 to 18 °C.
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Effects of Bafilomycin A1 and Methylamine HCl on Transcytosis of BoNT/A-- Bafilomycin A1 and methylamine HCl block toxin action at the nerve ending by inhibiting pH-induced translocation of the molecule from endosomes to the cytosol (20, 30, 31). Therefore, these drugs were examined for their effects on toxin movement across T-84 cells. Table II summarizes data from transcytosis experiments performed with bafilomycin A1 or methylamine HCl. Preincubation and assay in the presence of either of the agents resulted in a small yet significant (p < 0.01) decrease in the rate of transcytosis (Table II). Neither bafilomycin A1 (22% decrease) nor methylamine HCl (17% decrease) completely inhibited toxin transport across gut cells.
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Autoradiography of Transcytosed Toxin-- The work thus far indicates that polarized intestinal epithelial cells are capable of binding, transcytosis, and release of BoNT; however, this work does not answer two critically important questions. First, is the toxin that is transcytosed by T-84 or Caco-2 cells intact? Second, is the toxin that is transported across cells and delivered on the serosal side in a conformation that can evoke toxicity? The answer to the first question was obtained by iodinating homogeneous BoNT/A, then monitoring the binding, transcytosis and delivery of this material in T-84 and Caco-2 cells. The toxin molecule was examined: (a) prior to its addition to cells, (b) in a cytosolic fraction obtained from exposed cells, and (c) in the lower chamber after transcytosis across cells.
The results illustrating the state of both the starting material and that which was processed by cells are shown in Fig. 5, A and B. In A, lanes 1 (nonreducing) and 3 (reducing) show the toxin complex from which homogeneous toxin was purified, and lanes 2 (nonreducing) and 4 (reducing) show the purified toxin that was iodinated for transcytosis studies. An autoradiogram of iodinated BoNT/A that was added to the upper chamber for transcytosis studies is shown in B, lane 1 (reducing). Lane 2 (reducing) is an autoradiogram derived from the cytosolic fraction of exposed T-84 cells. Lane 3 (nonreducing) and lane 4 (reducing) are autoradiograms of the material delivered by these cells to the lower chamber. Note that the heavy chain and light chain components of the toxin recovered from the cytosol and from the basolateral side of T-84 cells were indistinguishable from those added to the cells. Also note that transcytosed toxin is not reduced during transit (B, lane 3). In B, lane 5 is an autoradiogram of iodinated toxin that was bound, transcytosed, and delivered to the basolateral side of Caco-2 cells. Once again, the heavy and light chain components of the toxin processed by the cells were indistinguishable from those added to cells.
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In Vivo and in Vitro Toxicity of Transcytosed Toxin-- To ensure that toxin delivered to the basolateral side of cells retained the ability to poison neuromuscular transmission, two types of bioassay were performed: in vivo toxicity experiments with mice, and in vitro toxicity experiments with isolated mouse phrenic nerve-hemidiaphragm preparations. For in vivo bioassay, animals were injected with an aliquot of medium collected from the lower well of T-84 cultures that were exposed to BoNT/A and monitored for toxicity for 12 h. This aliquot of medium (equivalent to ~50 ng of neurotoxin/animal, as calculated on the basis of experimental rates reported above; also see "Experimental Procedures") was diluted in phosphate-buffered saline-bovine serum albumin and administered intraperitoneally. All of the animals in this group died in an average of 255 ± 20 min (~4 h). This time frame is equivalent to that obtained when 50 ng of native, nontranscytosed toxin was used (data not shown). An equivalent volume of medium (see above) collected from the bottom of T-84 cells exposed to BoNT/C was not toxic to animals (none dead at 12 h), nor was an equivalent volume of medium collected from the lower well of MDCK cultures exposed to BoNT/A (none dead at 12 h). The results obtained in the animal bioassay are in line with expectations based on binding and transcytosis data presented earlier.
Data obtained for in vitro experiments confirmed that medium collected from the lower wells of T-84 cultures exposed to BoNT/A contained toxin that was able to paralyze an isolated neuromuscular junction. Aliquots of transcytosed toxin equivalent to ~1.0 µg of neurotoxin, calculated on the basis of experimental rates reported earlier (see above), were added to a 40 ml of organ bath. The resulting paralysis time was 56 ± 8.4 min. This time is equivalent to paralysis times recorded when 1.0 µg of native toxin was added to organ baths. Thus, comparison of data obtained with transcytosed toxin to data obtained for equivalent concentrations of native toxin demonstrated that transcytosed toxin retained full biological activity.Uptake of Toxin-associated Proteins by Differentiated T-84 and MDCK Cultures-- Botulinum toxin type A ordinarily occurs as part of a complex in which it is noncovalently associated with two other major proteins: a family of hemagglutinins (92, 57, 35, 21.5, and 17 kDa), and a nontoxic, nonhemagglutinating protein that shares some homology with neurotoxin (~120 kDa). Therefore, experiments were done to determine whether these proteins enter cells (viz. bulk-phase endocytosis) or are actively carried across cells (viz. transcytosis).
The associated proteins were iodinated identically to BoNT/A, then added to the upper wells bathing T-84 cells. The concentration of protein (10
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DISCUSSION |
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Botulinum toxin is an unusually potent substance that produces a type of food poisoning known as botulism. To produce its poisoning effects, the toxin must proceed through two separate and essential sequences of events. Initially, ingested toxin must traverse the gastrointestinal system and be absorbed into the general circulation. Subsequently, toxin must diffuse to peripheral cholinergic nerve endings, where it is internalized to produce blockade of exocytosis. The fact that the toxin is so potent means that both of these sequences of events must occur with a high degree of efficiency.
There is now a significant literature pertaining to binding and endocytosis of BoNT at the cholinergic nerve ending (see Introduction). This is in sharp contrast to the literature on toxin transport in the gut, for which there is almost a complete absence of work on cellular, subcellular, and molecular mechanisms. Therefore, the present study was undertaken with the goal of trying to identify an efficient mechanism by which intact and biologically active toxin could move from the mucosal to the serosal side of gut cells.
Experiments were conducted on two human cell lines of intestinal origin (T-84 and Caco-2), as well as a canine cell line of renal origin (MDCK). The results of this work support three conclusions: 1) human gut cells can bind and transport certain clostridial neurotoxins, 2) the toxins that are transcytosed are the same ones that are associated with human illness due to oral poisoning, and 3) the ability to bind and transcytose BoNT is not a generalized property of all differentiated and polarized cells that form tight junctions.
There are several routes in vivo that BoNT could exploit to enter the general circulation and ultimately reach the peripheral nervous system. First, there could be binding and transctyosis by intestinal epithelial cells. Second, there could be binding to M cells of Peyer's patches (32), presentation to the lymphatic system, and subsequent escape into the blood. And finally, the toxin could injure cells or disrupt tight junctions (33, 34), which would then permit nonspecific penetration of the gut. The work presented in this study was designed to test the possibility of binding and transcytosis by epithelial cells, but it did not rule out the possibility of involvement by M cells. For those serotypes that were transported (BoNT/A and BoNT/B), there was no evidence for loss of integrity of cellular membranes or tight junctions.
Iodinated BoNT/A was actively transported across differentiated and
polarized T-84 cells. Passive mechanisms such as diffusion between
cells did not appear to play a significant role, as judged by the study
of inulin flux. In cells that had formed tight junctions, the movement
of inulin from one cell surface to the other was greatly impeded. Given
that inulin (13 Å radius) is approximately 30-fold smaller in
molecular weight and 50-fold smaller in size than BoNT/A (48 Å radius)
(35), and given that T-84 junctional strands are essentially
impermeable to molecules with radii 5 Å (20), one can deduce
that passive diffusion of BoNT is likely to be negligible.
There were several observations that support the conclusion that movement of toxin across T-84 cells was an active process. First, labeled BoNT/A was capable of binding to T-84 cells, and this binding was significantly reduced in the presence of a molar excess of unlabeled toxin. This result suggests that the transport process begins with a specific binding step. Next, movement of toxin was greatly retarded when cells were incubated at low temperature, which indicates that the transport process was energy-dependent. Finally, movement of toxin was altered by drugs that have previously been shown to modify transcytosis, such as brefeldin A and nocodazole. When taken collectively, these data offer strong support for the belief that human intestinal cells can bind and transcytose BoNT.
Both in vivo and in vitro toxicity experiments showed that toxin delivered to the serosal side of cells was intact and biologically active. Thus, when toxin was added to the upper chamber of the Transwell® apparatus and aliquots of medium were recovered from the lower chamber, subsequent injection of the aliquots produced toxicity in mice that was identical to that produced by native toxin. Similarly, addition of aliquots from the lower chamber to in vitro tissue baths with phrenic nerve-hemidiaphragm preparations led to blockade of neuromuscular transmission. These data from toxicity experiments were in keeping with results from SDS-polyacrylamide gel electrophoresis gels, in which toxin recovered from the basolateral side of cells migrated identically to native toxin. The combined data show that human intestinal cells can bind and transcytose toxin in a form that is structurally and functionally intact.
It is interesting to note that the literature already has a number of studies that demonstrate transcytosis of intact proteins across intestinal epithelial cells (36-40), and in some cases the studies report rates of transcytosis (29, 41-43). The rate of transcytosis of BoNT/A determined in the present study is within the range of that reported for other proteins, but it is at the low end of the range. In this context, some recent preliminary experiments may prove to be important. It has been found that the rate of transcytosis of native unlabeled toxin is greater than that of iodinated toxin.2 Therefore, work is underway to determine whether iodination hinders binding, transcytosis, or release of BoNT.
There is highly suggestive evidence that the phenomenon of BoNT transcytosis described in this report is relevant to oral poisoning by the toxin. Epidemiology studies on human adults indicate that certain clostridial neurotoxins are associated with human illness caused by ingestion of toxin (e.g. BoNT/A and BoNT/B), whereas others are not (e.g. BoNT/C and tetanus toxin). It is interesting that this is precisely the same pattern one observes in the ability of human intestinal cells to bind and transcytose toxins. BoNT/A and BoNT/B were transported across T-84 and Caco-2 cells, but BoNT/C and tetanus toxin were translocated at much lower rates. This coincidence of patterns suggests that the relative absence of foodborne BoNT/C and tetanus toxin poisoning is due to the relative inability of these clostridial neurotoxins to penetrate from the gut to the general circulation.
The results with BoNT/C are particularly revealing. In a recent study, the actions of several botulinum toxins were studied on surgically excised and viable human neuromuscular junctions (23). This work demonstrated that human tissues are fully sensitive to the neuromuscular blocking properties of BoNT/C. Furthermore, experiments on cloning, sequence analysis and expression of human syntaxin showed that this peptide was a substrate for BoNT/C (23, 44). When the results of the earlier study on human nerves are combined with the results of the present study on human intestinal cells, they add to the argument that the relative absence of an efficient transcytosis mechanism in the gut may be adequate to explain the absence of human disease due to BoNT/C.
It is important to mention that movement of toxin across intestinal cells was clearly different from movement in MDCK cells or cholinergic nerve cells. In relation to MDCK cells, there was no evidence for significant binding and transcytosis. Apparently epithelial cells that form tight junctions are not universally capable of transporting toxin. In relation to cholinergic cells, previous work has shown that nerve endings internalize toxin by receptor-mediated endocytosis. Toxin then escapes endosomes by pH-induced translocation. Thus, drugs such as bafilomycin A1, which prevents acidification of endosomes, and methylamine HCl, which neutralizes acidification of endosomes, are potent blockers of translocation and toxin action (22, 30, 31). Neither of these drugs had a major effect on transcytosis of toxin in gut cells.
It should also be mentioned that, regardless of cell type, the fact that a protein was endocytosed was not necessarily an indication that it was efficiently transcytosed. Thus, BoNT/A underwent specific binding, endocytosis, and eventual transport across T-84 cells. In contrast, toxin-associated proteins such as hemaglutinin were endocytosed by T-84 cells, but only a small fraction of this material was transcytosed.
In conclusion, this study represents the first demonstration of transcytosis of biologically relevant concentrations of BoNT through a polarized epithelial cell layer consisting of differentiated intestinal cells that had formed tight junctions. The results of this work shed light on a likely mechanism by which toxin crosses human gut cells, and furthermore may explain why humans are sensitive to certain toxin serotypes but resistant to others. Beyond this, the findings raise exciting possibilities suggesting that BoNT binding and transcytosis could be exploited to create oral vaccines (45) or be used as a carrier for heterologous molecules. Experiments to test this hypothesis are currently underway.
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ACKNOWLEDGEMENTS |
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We thank Dr. James Madara and Rachel Kerner for sharing information on growth, maintenance, and differentiation of T-84 cells, Dr. Bibhuti DasGupta for providing a sample of toxin-associated hemagglutinins and guidance in purification of BoNT/A, and Dr. Nabil Bakry for assistance during toxin purification.
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FOOTNOTES |
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* This study was supported in part by National Institutes of Health NINDS Grant NS-22153 (to L. L. S.).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
To whom correspondence should be addressed: Rm. 314, Jefferson
Alumni Hall, Jefferson Medical College, 1020 Locust St., Philadelphia, PA 19107. Tel.: 215-955-8381; Fax: 215-955-2169; E-mail:
lance.simpson{at}mail.tju.edu.
The abbreviations used are: BoNT/A, botulinum neurotoxin serotype A; Caco-2, human colon adenocarcinoma; MDCK, Madin-Darby canine kidney; T-84, human colon carcinoma.
2 A. B. Maksymowych and L. L. Simpson, unpublished results.
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REFERENCES |
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