(Received for publication, July 9, 1996, and in revised form, October 24, 1996)
From the Veterans Administration Medical Center, Long Beach,
California 90822,
University of California School of
Medicine, Irvine, California 92717, § Center for Human Cell
Biotechnology, The University of Texas Health Science Center, San
Antonio, Texas 78284, and the ¶ University of Illinois and
Westside Veterans Administration Medical Center,
Chicago, Illinois 60612
A significant proportion of the bacterially synthesized folate in the large intestine exists in the form of folate monoglutamate. Recent studies in our laboratory using human colonic apical membrane vesicles have shown the existence of an efficient carrier-mediated system for folate uptake. Nothing, however, is known about the cellular regulation of the colonic uptake process. In this study, we used a recently established human normal colonic epithelial cell line NCM460 to address this issue. Uptake of folic acid by NCM460 cells was: 1) linear with time for 4 min of incubation and occurred with minimal metabolic alterations, 2) temperature- and pH- (but not Na+) dependent, 3) saturable as a function of concentration (apparent Km of 1.4 µM), 4) inhibited by structural analogs and anion transport inhibitors, and 5) energy-dependent. These characteristics of folic acid uptake by NCM460 cells are similar to those seen with apical membrane vesicles derived from human native colonic tissue. Using these cells, we found that protein kinase C- and Ca2+/calmodulin-mediated pathways have no role in regulating folic acid uptake. On the other hand, cAMP (through a mechanism independent of protein kinase A) and protein-tyrosine kinase-mediated pathways were found to play a role in the regulation of folic acid uptake by these cells. These results establish the suitability of NCM460 cells as an in vitro model system for investigating the details of the mechanism of colonic folate uptake and its regulation. Folic acid uptake by these cells appears to involve a carrier-mediated system, which is temperature-, pH-, and energy-dependent and appears to be under the regulation of cAMP and protein tyrosine kinase.
Folate is an essential micronutrient, which acts as a coenzyme in the synthesis of DNA and RNA and the interconversion and degradation of several amino acids (1-4). An adequate supply of folate is therefore necessary for normal cellular function, growth, and development. Folate deficiency has been suggested as one of the most common vitamin deficiencies in the Western Hemisphere (5, 6). Humans and other mammals cannot synthesize folate and rely on exogenous sources to meet their metabolic requirements. Folates are presented to the host from the diet and are also synthesized in the large intestine by normal microflora. The mechanism of absorption of dietary folate has been intensively examined over the past two decades at the tissue, cellular, subcellular, and more recently, molecular levels (6-15). Absorption of dietary folate has been shown to occur mainly in the proximal small intestine and involves a specialized, carrier-mediated system (6-12).
As to the bacterially synthesized folate in the large intestine, a significant amount of that folate exists in the monoglutamate, i.e. the absorbable form. Using [3H]p-aminobenzoic acid to label the newly synthesized folate by the intestinal flora, Rong et al. (16) have shown that a portion of this folate is indeed absorbed by the rat and is incorporated into its various tissues. Very limited studies, however, are available describing the mechanism and regulation of folate uptake by the colonocytes. Addressing this issue is of physiological importance because the colon has a unique structure, luminal environment, absorption mechanisms, and energy metabolism when compared with the small intestine. Folate uptake may also be of nutritional importance especially under conditions of massive disease or extensive resection of the small intestine (17-20). Furthermore, studies of folate metabolism at the cellular level may help clarify the causes of the localized folate deficiency believed to be associated with premalignant changes in colonic epithelia (21, 22).
Prompted by the above and the recent observation in our laboratory that a mRNA species from a mouse colon hybridizes with cDNA of a recently cloned folate carrier from mouse small intestine (the intestinal folate carrier-1) (14), we performed a study to directly test for a folate transporter in the colon. Using purified apical membrane vesicles prepared from human colonic tissue, we demonstrated the existence of an efficient carrier-mediated system for folate uptake that is pH-dependent and DIDS1-sensitive (23). Nothing, however, is known about the intracellular regulation of the folate uptake process in the colon. Studies with colonic apical membrane vesicles cannot provide such information because these structures lack the intracellular components. A colonic cell line that possesses a folate uptake mechanism that is similar to that of the native colonocyte would be an ideal model system to address this issue. The NCM460 cells (a normal, non-transformed epithelial cell line derived from the human transverse colonic mucosa) (24) were chosen as a model system because they possess characteristics similar to those of normal colonic epithelia (24, 25). In this report, we demonstrated that the mechanism of folate uptake is similar to that of the native colonic tissue and that the intracellular regulation of folate uptake is mediated by cAMP and PTK-mediated pathways. This is the first study of folate metabolism with in vitro cultured normal human colon cells.
[3H]Folic acid (specific activity, 30 Ci/mmol; radiochemical purity, >97%) was purchased from American Radiolabeled Chemicals (St. Louis, MO). [3H]Biotin (specific activity, 46.8 Ci/mmol) was obtained from DuPont NEN. Trypsin and other cell culture ingredients were from Sigma. All other chemicals were of analytical grade and were purchased from commercial sources.
The human normal colon epithelial cell line NCM460 was propagated to maintain its colonocyte features (24) in the culture medium M3:10TM (INCELL Corp., San Antonio, TX). The M3:10TM medium is M3TM base medium supplemented with 10% (v/v) fetal bovine serum and antibiotics and contains many growth factors and nutrients, some of which have been described elsewhere (26-28). NCM460 cells were used between passage 36 and 48 for this study. The cells were grown in 75-cm2 plastic flasks (Costar) at 37 °C in a 5% CO2 + 95% air atmosphere with media changes every 4 days. NCM460 cells were subcultured by trypsinization with 0.05% trypsin and 0.9 nM EDTA in Ca2+- and Mg2+-free phosphate-buffered saline solution and plated onto 12-well plates at a concentration of 5 × 105 cells/well. Uptake of folic acid was studied 3-6 days following confluence. Preliminary experiments showed no difference in folic acid uptake by NCM460 cells between day 3 and 12 postconfluence (data not shown). Cell growth was observed by periodic monitoring with an inverted microscope. Cell viability was tested by the trypan blue dye exclusion method and found to be >95%.
Uptake experiments were performed at 37 °C, unless otherwise mentioned. The incubation buffer was Krebs-Ringer phosphate buffer containing (in mM): 123 NaCl, 4.93 KCl, 1.23 MgSO4, 0.85 CaCl2, 5 glucose, 5 glutamine, 10 HEPES, and 10 MES, pH 5.0 (unless otherwise stated). [3H]Folic acid was added to the incubation buffer at the beginning of the experiment, and uptake was terminated after 3 min of incubation (unless otherwise specified) by the addition of 1 ml of ice-cold buffer followed by immediate removal by aspiration. The monolayers were rinsed twice with ice-cold buffer and digested with 1 ml of 1 N NaOH, neutralized by HCl, and then counted for radioactivity in a liquid scintillation counter. Protein contents of cell digests were estimated on parallel wells by the method of Lowry et al. (29) with bovine serum albumin used as the standard. Data presented in this paper are mean ± S.E. of multiple separate monolayers performed on at least two different occasions and are expressed in picomoles or femtomoles/mg of protein/unit of time. p values were calculated using the Student's t test. Kinetic parameters of folic acid uptake, i.e. maximal velocity (Vmax) and the apparent Michaelis constant (Km), were calculated using a computerized model of the Michaelis-Menten equation as described by Wilkinson (30).
Mechanism of Folic Acid Uptake by NCM460 Cells
Uptake with Time and Effect of Incubation TemperatureFig.
1 shows the time-dependent uptake of low
(5.4 nM) and high (3 µM) concentrations of
folic acid by NCM460 cells. In both cases the uptake was found to be
linear with time for up to 4 min of incubation and occurred at a rate
of 0.021 and 0.53 pmol/mg of protein/min for low and high
concentrations, respectively. Based on these results, 3 min of
incubation was chosen as the standard incubation time for all
subsequent experiments.
In a separate study, we examined the effect of incubation temperature on the uptake of folic acid (5.4 nM). Uptake was found to be significantly (p < 0.01) higher at 37 °C compared with uptake at 4 °C (61 ± 2 (n = 6) and 23 ± 1 (n = 6) fmol/mg of protein/3 min, respectively).
We also examined the metabolic form of the radioactivity taken up by NCM460 cells following 3 and 15 min of incubation with [3H]folic acid (21.6 nM). In this experiment cells were quickly washed at the end of incubation with ice-cold buffer, suspended in 50% water/methanol solution as described previously (10), homogenized, and then centrifuged. The supernatant was then applied to cellulose-precoated thin layer chromatography plates. The plates were run using a solvent system of 0.1 M anhydrous Na2HPO4 solution (pH 7.0). The results showed that 97.6 and 89.4% of the 3H radioactivity taken up by the monolayers to be in the form of intact [3H]folic acid after 3 and 15 min of incubation, respectively.
Role of Na+ and the Effect of Incubation Buffer pHThe role of Na+ in folic acid uptake by NCM460 cells was investigated in this study. This was done by examining the effect of iso-osmotically replacing Na+ (123 mM) in the incubation buffer with chloride salts of other monovalent cations such as K+ and choline (123 mM) or with the non-ionic mannitol (246 mM) on the uptake of folic acid (5.4 nM). The results showed no significant change in folic acid uptake under all conditions tested (56 ± 1 (n = 5), 57 ± 2 (n = 5), 52 ± 1 (n = 5), and 56 ± 6 (n = 5) fmol/mg of protein/3 min for control (Na+), K+, choline, and mannitol, respectively).
In a separate experiment we examined the effect of varying the
incubation buffer pH over the range of 3.5-8.5 on the uptake of folic
acid (5.4 nM). The results showed an increase in folic acid
uptake with decreasing incubation buffer pH with maximum uptake around
pH 5 (Fig. 2). Thus, we chose the buffer of pH 5 for all
other studies.
Uptake of Folic Acid as a Function of Concentration
Uptake of
folic acid uptake by monolayers of NCM460 cells was examined as a
function of increasing the substrate concentration in the incubation
medium. Uptake was found to include a saturable component at low
concentrations and to be linear at high concentrations. Uptake by the
saturable component was determined by subtracting uptake by diffusion
from the total uptake at each concentration (Fig. 3)
(uptake by diffusion was determined from the slope of the linear uptake
at high folic acid concentrations). Kinetic parameters of the saturable
uptake process were then determined as described under "Materials and
Methods" and found to be 1.4 ± 0.2 µM for the
apparent Km and 9.7 ± 0.6 pmol/mg of protein/3
min for the Vmax.
Effect of Unlabeled Folic Acid and Folate Structural Analogs on the Uptake of [3H]Folic Acid
The effect of unlabeled folic acid and the related structural analogs (5-formyltetrahydrofolate, 5-methyltetrahydrofolate, and methotrexate) on the uptake of 5.4 nM [3H]folic acid by NCM460 cells was examined in this study. Unlabeled folic acid and its related compounds (at 1 µM) caused significant inhibition (p < 0.01 for all) in the uptake of 5.4 nM [3H]folic acid (79 ± 2 (n = 6), 22 ± 1 (n = 6), 30 ± 3 (n = 6), 26 ± 1 (n = 6), and 34 ± 1 (n = 6) fmol/mg of protein/3 min for control and the presence of unlabeled folic acid, 5-formyltetrahydrofolate, 5-methyltetrahydrofolate, and methotrexate, respectively). The inhibition constant (Ki values) was then calculated using the Dixon method and found to be 1.1, 1.9, and 1.8 µM for 5-formyltetrahydrofolate, 5-methyltetrahydrofolate, and methotrexate, respectively.
Effect of Metabolic and Membrane Transport Inhibitors and Short Chain Fatty AcidsThe effect of the metabolic inhibitors sodium azide (10 mM) and 2,4-dinitrophenol (1 mM) and that of the sulfhydryl group inhibitor p-chloromercuriphenol sulfonate (1 mM) on the uptake of folic acid (5.4 nM) by NCM460 cells was examined in this study. Monolayers of NCM460 cells were preincubated with the above mentioned compounds for 30 min at 37 °C prior to uptake measurements. [3H]Folic acid was then added and incubation was continued for 3 min. All the compounds tested caused a significant inhibition (p < 0.01 for all) in folic acid uptake (70 ± 5 (n = 6), 20 ± 1 (n = 6), 17 ± 1 (n = 6), and 5 ± 1 (n = 6) fmol/mg of protein/3 min for control, sodium azide, 2,4-dinitrophenol, and p-chloromercuriphenol sulfonate, respectively).
In a separate experiment we examined the effect of 1 mM
anion transport inhibitors DIDS,
4-acetamido-4-isothiocyanostilbene-2,2
-disulfonic acid (SITS),
and probenecid on the uptake of folic acid (5.4 nM) by
NCM460 cells. The results showed significant inhibition
(p < 0.01) in folic acid uptake by all compounds
tested (81 ± 2 (n = 6), 16 ± 2 (n = 6), 25 ± 1 (n = 6), and
43 ± 3 (n = 6) fmol/mg of protein/3 min for
control, DIDS, SITS, and probenecid, respectively).
In another study we examined the effect of the short chain fatty acids, acetate, propionate, and butyrate (10 mM, sodium salt), in the incubation buffer on the uptake folic acid (5.4 nM) by NCM460 cells. The results showed that no significant change in the uptake of folic acid by NCM460 cells was observed in the presence of these anions compared with control (63 ± 2 (n = 4), 62 ± 2 (n = 4), 64 ± 3 (n = 4), and 61 ± 3 (n = 4) fmol/mg of protein/3 min for control, acetate, propionate, and butyrate, respectively).
Regulation of Folic Acid Uptake in NCM460 Cells and the Role of Protein Kinase-mediated Pathways
Following the determination of existence of a carrier-mediated system for folate uptake by NCM460 and the characterization of its nature, we examined possible regulation of the function of this carrier by specific protein kinase-mediated pathways. We focused on pathways that involve protein kinases for which consensus sequences have been shown to exist in recently cloned folate transporters (namely protein kinase C (PKC) and A (PKA)) (13-15, 31) and on pathways that have been shown to play a role in the regulation of uptake of other nutrients by intestinal and other epithelia (namely, PTK and Ca2+/calmodulin) (32-40).
The possible role of PKC in the regulation of folic acid uptake by NCM460 cells was tested by examining the effect of pretreating NCM460 cells for 1 h with either the PKC activator phorbol 12-myristate 13-acetate or with the PKC inhibitors bisindolylmaleimide or chelerythrine on the uptake of 5.4 nM folic acid. The results showed that none of these pretreatments significantly affected folic acid uptake (74 ± 9 (n = 11), 68 ± 8 (n = 11), 69 ± 9 (n = 11), and 66 ± 9 (n = 11) fmol/mg of protein/3 min for control and 1, 10, and 100 µM phorbol 12-myristate 13-acetate-pretreated cells, respectively; 69 ± 2 (n = 6), 79 ± 7 (n = 6), 72 ± 9 (n = 6), and 68 ± 3 (n = 6) fmol/mg of protein/3 min for control and 1, 10, and 100 µM bisindolylmaleimide-pretreated cells, respectively; 70 ± 4 (n = 6), 64 ± 2 (n = 6), and 61 ± 9 (n = 6) fmol/mg of protein/3 min for control, 2.5, and 25 µM chelerythrine-pretreated cells, respectively).
Involvement of PKA-mediated pathway in the regulation of folic acid uptake was also tested. This was done by examining the effect of pretreating NCM460 cells for 1 h with compounds that are known to increase intracellular cAMP levels (isobutylmethylxanthine (IBMX) and dibutyryl cAMP (Bt2cAMP)) and thus activate PKA and that of the specific PKA inhibitor H-89 on the uptake of 5.4 nM folic acid. The results showed that IBMX and Bt2cAMP cause a significant (p < 0.01) decrease in the uptake of folic acid. On the other hand H-89 did not cause any appreciable effect (Table I). We also examined the effect of pretreating cells with Bt2cAMP (1 mM) on folic acid (5.4 nM) uptake in the presence of H-89 (100 µM). No reversal in the inhibitory effect of Bt2cAMP by H-89 was observed (70 ± 4 (n = 4), 45 ± 2 (n = 4), 45 ± 1 (n = 4) fmol/mg of protein/3 min for the control, Bt2cAMP-treated, and both Bt2cAMP- and H-89-treated, respectively).
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In another study we tested for the involvement of PTK in the regulation of folic acid uptake by NCM460 cells. This was done by examining the effect of pretreating the NCM460 cells for 1 h with the PTK inhibitors genistein and tyrphostin A 25 on the uptake of 5.4 nM folic acid. Genistin and tyrphostin A 1, respectively, served as negative controls for these inhibitors. The results (Table II) showed that genistein (but not genistin) caused significant (p < 0.01) inhibition in folic acid uptake. Similarly, tyrphostin A 25 (but not tyrphostin A 1) caused significant (p < 0.01) inhibition in folic acid uptake (Table II). In contrast to the inhibitory effect of genistein on folic acid uptake by NCM460, genistein (50 µM) caused an increase in the uptake of the unrelated biotin (4.3 nM) (10 ± 1 (n = 3) and 40 ± 4 (n = 3) fmol/mg of protein/3 min for control and genistein-pretreated cells, respectively). We also examined the effect of genistein on the kinetic parameters of folic acid uptake by NCM460 cells. This was done by examining the effect of genistein (50 µM) on the uptake of folic acid as a function of concentration and comparing the results with that of control. The results showed that folic acid uptake was saturable both in the absence and presence of genistein; however, uptake in the presence of genistein was lower than that of control. Kinetic parameters were then calculated as described under "Materials and Methods." There was a decrease in the Vmax of folic acid uptake in genistein-pretreated cells compared with control cells (3.4 ± 0.8 and 9.7 ± 0.6 pmol/mg of protein/3 min, respectively), while the apparent Km was increased (2.9 ± 1.1 and 1.4 ± 0.2 µM, respectively). In a separate study we also examined the effect of pretreating (for 1 h) NCM460 cells with the tyrosine phosphatase inhibitor orthovanadate (100 µM) on the uptake of folic acid (5.4 nM). The results showed a significant (p < 0.01) increase in folic acid uptake by cells pretreated with orthovanadate (86 ± 4 (n = 4) fmol/mg of protein/3 min) compared with control (64 ± 5 (n = 4) fmol/mg of protein/3 min).
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The role of Ca2+/calmodulin-mediated pathways in the regulation of folic acid uptake by NCM460 cells was also tested. This was done by examining the effect of pretreating (for 1 h) these cells with the calmodulin inhibitors trifluoperazine, calmidazolium, and W13 and with the inhibitor of Ca2+/calmodulin kinase II, KN62, on the uptake of folic acid (5.4 nM). The results showed that none of these compounds cause a significant effect on folic acid uptake (63 ± 1 (n = 6), 66 ± 2 (n = 6), and 67 ± 3 (n = 6) fmol/mg of protein/3 min for control and 50 and 100 µM trifluoperazine-pretreated cells, respectively; 67 ± 2 (n = 6), 68 ± 3 (n = 6), 66 ± 3 (n = 6), and 62 ± 4 (n = 6) fmol/mg of protein/3 min for control and 10, 50, and 100 µM calmidazolium-pretreated cells, respectively; 50 ± 1 (n = 6) and 51 ± 1 (n = 6) fmol/mg of protein/3 min for control and 100 µM W13-pretreated cells, respectively; 50 ± 1 (n = 6) and 50 ± 1 (n = 6) fmol/mg of protein/3 min for control and 50 µM KN62-pretreated cells, respectively).
The major aim of the present study was to establish the
suitability of NCM460 cells as a model to study the details of colonic folate uptake mechanism and its cellular regulation. We chose this
normal non-transformed human colonic epithelial cell line because these
cells possess many of the characteristics of the native colonocytes
(24, 25). Our results showed that uptake of folic acid was
temperature-dependent and occurred with minimal metabolic
alterations to the transported substrate. Na+ in the
incubation medium appeared to play no role in folic acid uptake as
indicated by the lack of effect of Na+ removal on uptake.
On the other hand, incubation buffer pH (i.e. H+
concentration) appeared to play an important role in driving folic acid
uptake. Increasing the H+ concentration in the incubation
medium by lowering the incubation buffer pH led to a marked increase in
folic acid uptake. The effect of pH on folic acid uptake by NCM460
cells may represent the existence of a
folate/OH
exchange mechanism (or a
folate
/H+ cotransport) and/or represent a
direct effect of pH on the folate uptake carrier, as suggested before
(9, 11).
The uptake process of folic acid by NCM460 was saturable as a function of increasing the substrate concentration with an apparent Km and Vmax of 1.4 ± 0.2 µM and 9.7 ± 0.6 pmol/mg of protein/3 min, respectively. This finding indicates the involvement of a carrier-mediated system in the uptake process. This conclusion was further supported by the finding of a significant inhibition in [3H]folic acid uptake by unlabeled folic acid and by its structural analogs. The inhibition constants (Ki) for the folate structural analogs 5-formyltetrahydrofolate, 5-methyltetrahydrofolate, and methotrexate were 1.1, 1.9, and 1.8 µM, respectively. The finding that the Ki values of these analogs are similar to the apparent Km of the substrate (folic acid) transport suggests that these analogs share the same uptake mechanism with folic acid in NCM460 cells. The process of folic acid uptake by NCM460 cells was also energy-dependent as indicated by the significant inhibition in the uptake process by different metabolic inhibitors.
The folic acid uptake process was sensitive to the effect of the anion
transport inhibitors DIDS, SITS, and probenecid, further suggesting the
possible involvement of a folate/OH
exchange mechanism. Because (i) the process is sensitive to these anion
transport inhibitors and (ii) colonic lumen contains high concentrations of the anions acetate, propionate, and butyrate (31), we
also tested the effect of these short chain fatty acids on the
carrier-mediated uptake of folic acid by NCM460 cells. Our results,
however, showed that these anions have no effect on the uptake
process.
All of the above described characteristics of folic acid uptake mechanism by the NCM460 cell line are similar to those recently observed with purified apical membrane vesicles prepared from native human colonic tissue (23). This clearly establishes the suitability of this cell line as a model with which to study the cellular regulation of folate uptake by the human colon. Using these cells we then tested the possible involvement of specific protein kinase- and Ca2+/calmodulin-mediated pathways in the regulation of folic acid uptake by colonocytes. We focused on pathways that involve protein kinases (PKC and PKA) for which consensus sequences have been shown to exist in the recently cloned folate carriers (13-15, 32) as well as those pathways that have been shown to play an important role in the regulation of uptake of other nutrients by epithelial cells (PTK- and Ca2+/calmodulin-mediated pathways) (33-41). When specific modulators of these pathways were used, we found that PKC-mediated pathways had no role in regulating folic acid uptake by NCM460 cells. In contrast, compounds that increased the intracellular cAMP level, namely IBMX and Bt2cAMP, caused a significant decrease in folic acid uptake. However, the specific inhibitor of PKA H-89 had no significant effect on folic acid uptake, and when cells were pretreated with Bt2cAMP in the presence of H-89, the inhibitory effect caused by Bt2cAMP was not reversed. These findings suggested that intracellular cAMP affects folic acid uptake through a PKA-independent mechanism. Similar observations and conclusions were reported by Muller et al. (42) in their findings on the inhibition of the H+/peptide cotransporter by intracellular cAMP level in the human intestinal epithelial cell line Caco-2. Assuming that the expressed folate carrier in NCM460 cells is similar to the recently cloned folate carriers in that it has consensus sequences for PKC and PKA, our findings may suggest that either phosphorylation of these sites has no effect on the function of the folic acid uptake carrier or that these consensus sites are not accessible to these protein kinases.
Although the regulation of folic acid uptake by NCM460 cells was apparently not mediated by the PKC- and PKA-mediated pathways, a role for the PTK-mediated pathway was suggested by the observations that inhibitors of PTK activity, namely genistein and tyrphostin A25, caused a significant decrease in folic acid uptake. The effect of these compounds appeared to be specific because their negative controls (genistin and tyrphostin A1, respectively) did not affect folic acid uptake. Furthermore the uptake of the unrelated biotin was up-regulated by genistein. The inhibitory effect of genistein appeared to be mediated through a decrease in the Vmax of the folic acid uptake process and an increase in the apparent Km. These findings suggest that the inhibitory effect caused by genistein is mediated through a decrease in the affinity, activity, and/or number of the folic acid uptake carriers. The ability of the PTK phosphatase inhibitor orthovanadate to cause a significant increase in folic acid uptake further supports the suggested involvement of PTK in the regulation of folic acid uptake by NCM460 and raised the possibility that phosphorylation may be involved. It should be mentioned here, however, that the sequences of the folate carriers cloned so far contained no consensus sites for PTK phosphorylation. Our findings, therefore, may suggest that a "cryptic" rather than a consensus ("canonical") site(s) for PTK phosphorylation may be involved in the regulation of folate transport. Alternatively the possibility that PTK is acting on an auxillary protein, which then exerts its effect on the folic acid uptake carrier, cannot be ignored. Further studies are needed to address these issues. Similar findings have been reported in the case of the rat renal Na/Pi cotransporter clone where no consensus sites for PKA phosphorylation were found in the cloned carrier, yet transport activity is regulated by a PKA-mediated pathway (43). Further, PKC-mediated inhibition of the rat renal Na/Pi cotransporter was not prevented by the removal of the protein kinase C consensus sequences (44). Similarly, a cryptic site for PKC has been identified at the amino terminus of the Na+/K+-ATPase (45).
In summary, our results demonstrate the suitability of the NCM460 cell line as an in vitro model system to investigate the detailed mechanism and regulation of folic acid uptake by colonocytes. Uptake appears to be via a carrier-mediated system which is temperature-, pH- and energy-dependent and appears to be under the regulation of PTK and cAMP. Regulation of folate uptake by PTK and cAMP may suggest that the process is under the influence of growth factors and other biologically active agents. Further studies are needed to address this issue.
We thank Lawrence A. Manzano for technical assistance and Drs. David Dyer and Taoi Nguyen for helpful discussions.