Colitis-Induced Changes in the Expression of the Na+/H+ Exchanger Isoform NHE-1

QUICK SEARCH:

[advanced]

	Author:		Keyword(s):
Year:		Vol:		Page:

This Article

	Abstract
	Full Text (PDF)
	Submit a response
	Alert me when this article is cited
	Alert me when eLetters are posted
	Alert me if a correction is posted
	Citation Map

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via Google Scholar

Google Scholar

	Articles by Khan, I.
	Articles by Abul, H.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Khan, I.
	Articles by Abul, H.

Vol. 285, Issue 2, 869-875, May 1998

Colitis-Induced Changes in the Expression of the Na⁺/H⁺ Exchanger Isoform NHE-1

Islam Khan, Farida M. Al-Awadi and Habib Abul

Department of Biochemistry (I.K., F.M.A-A.) and Department of Pharmacology (H.A.), Faculty of Medicine, Kuwait University, Kuwait

	Abstract

Top Abstract Introduction Materials & Methods Results Discussion References

The sodium hydrogen exchanger (NHE) plays an important role in the absorption of NaCl, the regulation of intracellular pHand cell growth. These functions are compromised in the inflammatorybowel diseases. The objective of this study was to examine theexpression of the NHE-1 isoform during colitis induced by aceticacid or trinitrobenzenesulfonic acid in Sprague-Dawley male rats.We also examined the effect of dexamethasone on the expressionof NHE-1. Levels of mRNA were estimated using the reverse transcription-polymerasechain reaction and slot blot analysis, and levels of protein wereestimated by enhanced chemiluminescence light Western blot analysis.The levels of the NHE-1 mRNA and protein in colonic mucosa increasedas assessed at 1, 2, 5 and 7 days post-acetic acid administrationand 7 days post-trinitrobenzenesulphonic acid administration inthe rats. The levels of mRNA were not suppressed by dexamethasonetreatment in either case. These findings demonstrate that colitis-inducedexpression of the NHE-1 mRNA and protein is independent of theway colitis is induced. Although factor(s) responsible for theinduction remain to be identified, our findings showing similarchanges in the NHE-2 and NHE-3 mRNA isoforms, together with thelack of their suppression by dexamethasone, suggest that cytokinesand intracellular pH are secondary factors.

	Introduction

Top Abstract Introduction Materials & Methods Results Discussion References

NHE transports extracellular Na⁺ for intracellular H⁺ electroneutrally and is present in every mammalian cell (Bianchini andPouyssegur, 1995; Noel and Pouyssegur, 1995). Recent studies havedemonstrated four different genes encoding the isozymes NHE-1,NHE-2, NHE-3 and NHE-4 (Bookstein et al., 1994; Collins et al.,1993; Orlowski et al., 1992; Wang et al., 1993). These isoformsexhibit differential distribution in the GI tract. The NHE-1 isoformis located on the basolateral side of the epithelial cell andis considered a main regulator of pH_i and cell volume, whereasthe apical isoforms NHE-2 and NHE-3 are known to regulate NaClabsorption (Levine et al., 1993; Maher et al., 1997; Tse et al.,1992). These isoforms differ in their sensitivity to amilorideand in their regulation by hormones and growth factors (Bianchiniand Pouyssegur, 1995; Noel and Pouyssegur, 1995; Tse et al., 1992;Tse et al., 1993).

Intestinal epithelial cells act as an important site of absorption of the luminal contents. They are also the primary targetof insults that cause IBDs. These cells actively participate ininflammatory reactions by producing cytokines, growth factors(Justinichi et al., 1992; Volker et al., 1995) or derivativesof arachidonic acid (Dias et al., 1992). These mediators alterthe membrane permeability and activity of ion-transporting proteinssuch as Na/K-ATPase during IBDs in human and in animal models(Allgayer et al., 1988; Khan and Collins, 1993; Wild and Murray,1989). In Crohn's disease, the pH_i of colonocytes is decreased(Rowe and Bobar, 1995). Because NHE-1 is the main regulator ofpH_i, cellular growth and differentiation, in the present studywe examined expression of the NHE-1 isoform. Animal models haveproved useful in understanding the underlying mechanisms of alteredphysiological functions. However, the changes seen during colitismay be influenced by the nature of the colitides as well. Therefore,in this study we investigated the mechanism of NHE-1 expressionin HAC- and TNBS-induced colitis. Further, to identify the factorsresponsible for the expression of NHE-1 during colitis, we alsoexamined the effect of dexamethasone on the NHE-1, NHE-2 and NHE-3levels of mRNA.

The specific aim of the present study was to investigate the underlying mechanism of NHE-1 expression during colitis inducedby HAC or TNBS. We employed the RT-PCR and slot blot analysisfor quantitation of the mRNA levels and the ECL Western blot analysisfor protein estimation.

	Materials and Methods

Top Abstract Introduction Materials & Methods Results Discussion References

Induction of colitis. Sprague-Dawley male rats weighing 230 to 280 g and maintained by the Faculty of Medicine, Kuwait University, were used inthis study. Colitis was induced by intrarectal administrationHAC (Grossi et al., 1993; Khan and Al-Awadi, 1997; McPherson andPfeiffer, 1977) or TNBS (Fluka Bucks, Switzerland) as described(Morris et al., 1989). Rats that received PBS and rats that received50% ethanol vehicle served as controls for HAC- and TNBS-inducedcolitis, respectively. Animals were sacrificed by cervical dislocationafter 1, 2, 5 and 7 days of HAC and after 7 days of TNBS administration.A colonic segment 6 cm long was taken from the site of inflammationand cleaned with sterile PBS. Mucosa was scraped off and storedfrozen at $-$ 70°C until use. The mucosal scrapping contained mucosaand submucosa from both the control and the inflamed colon. However,the tissue was not homogeneously pure because of the presenceof other cell types. The mucosal scrappings so obtained were usedin the experiments reported in this study. The rats were treatedi.p. with dexamethasone (1 mg/kg body weight) 2 h before HAC orTNBS administration, and the dose was repeated every 24 h. Onthe third day after HAC administration or on the seventh day afterTNBS administration, animals were sacrificed and tissues used.

MPO activity. MPO activity was estimated in the whole colonic tissue obtained from the rats (Bradley et al., 1982; Khan and Al-Awadi, 1997).MPO activity was estimated in the whole colonic segment containingmucosa and muscle layers. Tissue was taken from the site of inflammation,minced finely with scissors in (1 gm/10 ml) 50 mM potassium phosphatebuffer, pH 6.0, containing 14 mM hexadecyltrimethylammonium bromide(Sigma, UK). Tissues were homogenized with a polytron (Janke andKunkle Staufen, FRG) for 1 min. Lysates were frozen in liquidnitrogen and thawed once. The lysates were centrifuged for 2 minin cold room at 15,000 × g (Eppendorf). Supernatants were usedto estimate the MPO activity in the presence of o-dianisidine-HCl(Sigma, UK) and 0.0005% H₂O₂ (Khan and Al-Awadi, 1997). Opticaldensity was recorded at 415 nm every 15 s over a period of 1 minusing a spectrophotometer, DU700 (Beckman, CA). MPO activity wasexpressed as units per minute per milligram of tissue. The enzymeunit is defined as the conversion of 1 µmol H₂O₂/minute/mg oftissue at room temperature.

Extraction of total cellular RNA. RNA was extracted from the frozen colonic mucosa by the guanidinium isothiocyanate-cesium chloride centrifugation method (Chirgwinet al., 1979; Khan and Al-Awadi, 1997). Frozen colonic mucosa(1 g/10 ml) was thawed in 4 M guanidinium isothiocyanate (Sigma),minced finely with scissors and homogenized with the polytron.The homogenates were centrifuged at 10,000 × g (J2-MI, Beckman)at 4°C for 10 min. The supernatants were layered on 3.5 ml of5.7 M cesium chloride solution (Sigma) and centrifuged at 110,000× g for 24 h at 16°C using an SW41 rotor (LX-80 Beckman, CA).The pellet of RNA was dissolved in diethylpyrocarbonate (DEPC,Sigma)-treated and autoclaved distilled water and was extractedonce with phenol-chloroform. RNA was precipitated from the aqueouslayer with 2.5 vol of absolute ethanol for 2 h at $-$ 70°C (Khanand Al-Awadi, 1997). RNA was recovered by centrifugation of thesamples in cold room at 14,000 rpm (5415C Eppendorf) for 20 minand dissolved in the RNase-free water. The concentration of RNAwas determined spectrophotometrically at 260/280 nm. The qualityof RNA was routinely electrophoretically analyzed on a formaldehyde-agarose(1.4%) gel (Khan and Al-Awadi, 1997; Khan and Collins, 1993; Sambrooket al., 1989). All solutions and glassware were made RNase-freeby DEPC treatment followed by autoclaving. Heat-sensitive solutionswere made in RNase-free water and filtered subsequently througha 0.45-µm millipore filter.

RT. Aliquots (5 µg) of total RNA were mixed with 250 ng oligodT primer (Promega, WI) and heated at 75°C for 10 min. Annealingwas performed by slow cooling of the heated sample to 37°C (Khanand Al-Awadi, 1997; Khan et al., 1992). RT was carried out inthe presence of 15 to 20 units of AMV reverse transcriptase (Pharmacia,Uppsala, Sweden) and 15 units of RNA guard (Pharmacia, Uppsala,Sweden) using a buffer containing (mmol/l): 10 Tris-HCl, pH 8.4,at 42°C, 10 MgCl₂, 70 KCl, and 10 dithiothreitol for 30 min at37°C followed by a 30-min incubation at 42°C (Khan et al., 1992;Khan and Al-Awadi, 1997). The reverse reaction was terminatedby heating the samples at 90°C for 10 min. The cDNA so obtainedwas routinely employed for amplification of the NHE-1 mRNA isoformusing the specific primers (table 1). The primers were selectedon the basis of rat kidney, brain or stomach cDNA information(Orlowski et al., 1992). Whether there is an intron present inthe region between the primers is not known.

View this table:
[in this window]
[in a new window]

TABLE 1
Structure of the primers used
The structures of the primers used in this study, the size of the PCR fragment in base pairs and the corresponding reference are shown.

PCR. Aliquots (5 µl) of cDNA were routinely amplified by PCR using 1 to 2 units of Amplitaq (Perkin-Elmer, Norwalk, CT) and 50pmol of each primer (table 1). The conditions were optimized inthe linear range of amplification, in accordance with the basicPCR protocol described elsewhere (Innis et al., 1990; Khan andAl-Awadi, 1997; Khan et al., 1992). The following PCR conditionswere used: denaturation 94°C × 30 s; annealing 55°C × 30 s; extension74°C × 60 s. Aliquots (5 µl) of PCR products were analyzed electrophoreticallyusing a 7% polyacrylamide gel (Khan and Collins, 1993; Khan etal., 1992). The gels were stained with ethidium bromide and photographedon a gel documentation system (Stratagene, CA). To ensure thatthe PCR bands were not due to genomic contamination, two controlswere used, one containing RNA without RT and the other withoutcDNA or RNA.

Quantitation of mRNA. The area of the PCR band was obtained by scanning the negatives on a densitometer (Pharmacia LKB, UltroScan-XL), and the ratioNHE-1 mRNA:internal control, alfa-1 isoform of sodium pump (Khanand Collins, 1993) was calculated. OligodT primer was used forRT, and from the same cDNA sample, NHE-1 and internal controlwere amplified separately. This technique was chosen to minimizetube-tube variations during the reverse reaction.

Slot blot analysis. The RT-PCR data were validated using slot blot analysis. Aliquots of 20 µg total RNA were spotted on to the nitrocellulosefilter (Bio-rad, CA) using a slot blot apparatus (Bio-rad). RNAwas immobilized by heating the filters for 2 h at 80°C. The filterswere prehybridized for 2 h and hybridized with biotinylated downstreamprimer (Genosys, UK) listed in table 1. Hybridization was carriedout at 42°C in 5XSSC. Subsequently, the filters were washed with2XSSC buffer at 40°C and incubated with streptavidin-horseradishperoxidase (1:2000) for 1 h at ambient temperature. The filterswere washed with 2XSSC three times at ambient temperature. Signalswere developed using the ECL kit components 1 and 2 for 1 min.The autoradiogram was scanned on a densitometer to obtain thearea of the bands.

Western blot analysis. NHE-1 protein was measured using NHE-1 antibodies (a kind gift from Dr. E. B. Chang). Crude plasma membranes were preparedfrom mucosal scrapings, following the standard method with modifications(Shallat et al., 1996). Briefly, mucosal scrapings were homogenizedwith a polytron for 60 s in 250 mM sucrose and 20 mM MOPS buffer,pH 7.5, and centrifuged for 10 min at 450 × g at 4°C; the resultingsupernatant and pellet were designated supernatant 1 and pellet1. Pellet 1 was rehomogenized and centrifuged. The resulting supernatant1 and supernatant 2 were pooled and centrifuged at 20,000 × gin the JA20 rotor of a Beckman high-speed centrifuge for 45 minat 4°C. Supernatant was discarded and pellet 3 was collected.Pellet 2 was used to check the loss of the NHE-1 protein. Pellet3 was suspended in the sucrose-MOPS buffer and homogenized. Totalprotein was measured using a dye-binding assay kit (Bio-rad).Pellet 3 samples were used to measure the NHE-1 protein level.Aliquots containing 50 µg total protein from each sample wereseparated on a 7.5% polyacrylamide gel electrophoretically underdenaturing conditions (Laemmli, 1970) and transferred onto thenitrocellulose filter (Bio-rad) electrophoretically. Filters wereblocked with 5% nonfat dry milk in PBS for 2 h at ambient temperature.Antiserum of NHE-1 was added to the blocked filters, incubatedat ambient temperature for 2 h and washed thoroughly with PBS.Anti-rabbit secondary antibodies conjugated with horseradish peroxidase(Sigma) were added (1:5000) to the filters and incubated for 1h at ambient temperature. Subsequently, the filters were washedwith PBS and incubated with components 1 and 2 of the ECL kit(Amersham) for 1 min. The filters were exposed to X-ray film (Kodak)for 5 to 20 s, and the signals were developed. The bands werescanned on the densitometer to obtain the band area.

Analysis of data. The area of the bands was obtained by scanning the negatives on a densitometer (Pharmacia LKB, Uppsala, Sweden; UltroScan-XL).Statistical analysis was performed using the SPSS program. A valueof P < .05 was considered statistically significant.

	Results

Top Abstract Introduction Materials & Methods Results Discussion References

MPO activity. MPO activity is considered a reliable marker of inflammation; therefore, we estimated MPO activity to monitor colitis. MPOactivity increased in a time-dependent manner during 1, 2 and5 days (fig. 1) and returned to the basal level after 7 days ofHAC administration. MPO activity was also significantly higherafter 7 days of TNBS administration than in the control untreatedrats (fig. 2). MPO activity was suppressed significantly afterthe dexamethasone treatment of the HAC- or TNBS-induced colitis(fig. 2).

View larger version (17K):
[in this window]
[in a new window]

Fig. 1. Bar diagram showing MPO activity in the colon of rats that received HAC on the days indicated before assessment. Data are mean ± S.E.M. (n = 10). * P < .002.

View larger version (33K):
[in this window]
[in a new window]

Fig. 2. The MPO activity (hatched bars), NHE-1 mRNA measured by RT-PCR (open bars) and slot blot analysis (closed bars) in PBS (control), HAC (3 days after the administration of HAC), HD (3 days after the administration of HAC + dexamethasone), ET (ethanol control), TNBS (7 days after the administration of TNBS) and TD (7 days after the administration of TNBS + dexamethasone). Data are mean ± S.E.M. (n = 8). * P < .02 vs. controls.

Restriction analysis and sequencing. It was necessary to characterize the NHE-1 PCR fragment before estimating the mRNA level. Restriction endonucleases recognizespecific sequences in a DNA fragment, so the NHE-1 PCR fragmentwas identified using AvaII restriction enzyme. AvaII restrictionsites were identified using DNASIS software (Pharmacia) in thePCR fragment, which on digestion was expected to yield 7-, 49-,51-, 56- and 105-bp fragments. But we obtained only two bands;one probably contained 49-, 51- and 56-bp fragments migratingtogether (fig. 3, lane 2, lower band) and the other correspondedto 105 bp (fig. 3, lane 2, upper band). Because it was difficultto separate and match the size of 49, 51 and 56 bp of AvaII fragmentsaccurately, we further identified the NHE-1 PCR fragment by nucleotidesequencing using a nonradioactive method. The PCR fragment waspurified using a DNA purification kit (U.S. Biochemical) and sequenced.Briefly, 200 ng of the purified PCR-fragment was mixed with 3.2pmol of sense or antisense primer (table 1) and amplified (9600Thermocycler, Perkin-Elmer) using the fluorescent dye terminatorsand Taq DNA polymerase mix (Perkin-Elmer) for 40 cycles. The PCRconditions were denaturation 94°C × 30 s, annealing 50°C × 30s and extension 60°C × 90 sec. After amplification, the sampleswere extracted once with phenol-chloroform and dissolved in theloading buffer. The samples were run on an automated DNA sequencer(Applied Biosystems) and analyzed. The derived nucleotide sequenceshowed 100% identity with the published sequence (data not shown).

View larger version (56K):
[in this window]
[in a new window]

Fig. 3. Amplification of the NHE-1 PCR fragment (208 bp) in the colonic mucosa of the control rats (lane 1). The fragments resulting from the complete digestion of the 208-bp fragment with AvaII are shown in lane 2, upper bright band (105 bp) and lower band (49-56 bp). The unlabeled lane contains a 100-bp DNA ladder.

Yield of total cellular RNA. To rule out the possibility that differences in the yield of total RNA from the control and the inflamed colon contributeto the changes in the mRNA levels, we estimated total RNA. Theamount of total RNA (2.0 ± 0.25 mg/g) in the control rats didnot differ significantly from the amounts of RNA [(mg/g): 1.7± 0.20, 1.9 ± 0.17, 1.6 ± 0.20 and 1.5 ± 0.32] obtained from thecolonic mucosa of rats after 1, 2, 5 and 7 days of HAC administration,respectively. The quality of total RNA prepared each time wasroutinely analyzed (fig. 4A) electrophoretically using a 1.2%formaldehyde-agarose gel (Sambrook et al., 1989). The qualityof total RNA was consistent in all the samples, as shown by theintensity of the 28s and 18s ribosomal RNA bands (fig. 4A). Theyields of total RNA [(mg/gm tissue): 1.7 ± 0.20, 1.8 ± 0.15 and1.5 ± 0.14] from the rats that received PBS, ethanol and TNBS,respectively, were also not significantly different.

View larger version (50K):
[in this window]
[in a new window]

Fig. 4. Representative gel picture shows the quality of total RNA. RNA extracted from the control rats is shown in lane 1, and RNA from the rats that received HAC 1, 2, 5 and 7 days earlier is shown in lanes 2, 3, 4 and 5, respectively. Each lane contains 5 µg total RNA. The positions of 28s (upper arrow) and 18s (lower arrow) ribosomal RNAs are indicated (fig. 4A). Ethidium bromide-stained gel picture showing the PCR amplification of the NHE-1 (Figure 4B) and alfa-1 isoform (fig. 4C). NHE-1 mRNA levels estimated by slot blot analysis are shown in figure 4D. In each figure, the level of mRNA in the control rats is shown in lane 1, and the level of mRNA in the rats that received HAC 1, 2, 5 and 7 days earlier is shown in lanes 2, 3, 4 and 5, respectively. Lane 6 (fig. 4D) is a negative control, and the unlabeled lane (fig. 4B) contains the PBR322xHaeIII size marker. Each lane shows the level of PCR product in 250 ng of total RNA from colonic mucosa after amplifying for 21 cycles. Figure 4E shows that the percent increases calculated from the ratios NHE-1:SD by RT-PCR (closed bars) on the days indicated as post-administration of HAC were not significantly different from those calculated from slot blot analysis (hatched bars). Cycle-dependent amplification of the NHE-1 ( $bullet$ ) and sodium pump mRNA ( $open circle$ ). Data are mean ± S.E.M. of duplicate determinations (fig. 4F). Representative gel picture (fig. 4G) showing PCR amplification of the indicated isoforms of the NHE and internal control sodium pump (SD). Lanes 1 (control rats), 2 (rats that received HAC 3 days earlier) and 3 (dexamethasone treatment of the rats that received HAC 3 days earlier) contain equal amounts of total RNA as the starting material (fig. 4G).

Profile of NHE-1 mRNA. The basal level of NHE-1 (fig. 4B, lane 1) measured by RT-PCR increased in a time-dependent manner during 1, 2, 5 and 7 daysafter HAC administration (fig. 4B, lanes 2-5, respectively). Thelevel of alfa-1 RNA internal control decreased in the same samples(fig. 4C, lanes 2-5) as compared with the untreated control rats(fig. 4C, lane 1). Slot blot analysis (fig. 4D) also showed increasedlevels at 1, 2, 5 and 7 days (fig. 4D, lanes 2-5) after HAC administrationas compared with the control rats (fig. 4D, lane 1). Both methodsproduced comparable percent increases in the level of NHE-1 mRNA(fig. 4E). The PCR conditions were standardized in the linearrange of amplification of both NHE and sodium pump internal controlusing different cycle numbers in the presence of 2 mM MgCl₂ (fig.4F).

Similarly, during TNBS-induced colitis, the levels of NHE-1 mRNA in the control rats were elevated, and this effect was notsuppressed by dexamethasone treatment (fig. 2). Increases in NHE-1mRNA after 3 days of HAC administration were also not suppressedby dexamethasone treatment (fig. 2). We have previously showninduction of NHE-2 and NHE-3 mRNA due to colitis induced by HAC(Khan et al., 1996

). The effect of dexamethasone on the colitis-inducedelevation in NHE-2 and NHE-3 mRNA was examined in the presentstudy. The levels of NHE-2 (fig. 4G, lane 2) and NHE-3 mRNA (fig.4G, lane 2) were increased significantly in the HAC-inflamed colonas compared with the PBS control (fig. 4G, lane 1). The inductionof mRNA was not reversed by dexamethasone treatment (fig. 4G,lane 3) of animals that received HAC 5 days earlier. However,in both models of colitis, MPO activity was suppressed significantlyby dexamethasone (fig. 2).

Western blot analysis. To investigate whether changes seen at the mRNA level are also translated into protein, we estimated levels of the NHE-1 proteinby ECL Western blot analysis using NHE-1 antibodies raised inrabbit (a kind gift from Dr. E. B. Chang). Because dexamethasonedid not suppress the level of NHE-1 mRNA, we did not measure thelevels of the protein. The NHE-1 antibodies reacted with the 90-to 92-kD band corresponding to the size of the NHE-1 protein (fig.5A). The antibodies also showed some cross-reaction in colonicpreparations, but the reaction was more specific and intense withthe kidney positive control (fig. 5A). In the same amount of crudemembranes from colonic mucosa, the amount of NHE-1 protein increasedas assessed at 1, 2, 5 and 7 days after HAC administration (fig.5, A and B) as compared with the control rats. There was no lossof NHE-1 protein in pellet 2 (data not shown). Similarly, in anequal amount of crude membranes, the level of NHE-1 protein wasincreased in the colonic mucosa from rats that had colitis inducedby TNBS (fig. 6, A and B) as compared with the PBS or ethanolcontrol group.

View larger version (38K):
[in this window]
[in a new window]

Fig. 5. ECL Western blot analysis showing the NHE-1 protein in the crude membranes from control rats (lane 1) and from rats that received HAC 1 (lane 2), 2 (lane 3), 5 (lane 4) and 7 (lane 5) days earlier. Lane 6 shows NHE-1 from the kidney microsomes positive control. Each lane contains 50 µg of crude membrane proteins. Position of NHE-1 is shown. Bar diagram showing (on the y-axis) a time-dependent increase in the NHE-1 protein levels (band area) in rats that received HAC 1 (bar 1), 2 (bar 2), 5 (bar 5) and 7 (bar 7) days earlier as compared with control rats (bar 0) shown on the x-axis. Data are mean ± S.E.M. (n = 6, P < .04).

View larger version (40K):
[in this window]
[in a new window]

Fig. 6. ECL Western blot analysis showing the NHE-1 protein levels (band area) in the mucosal crude membranes (50 µg) from rats that received PBS (lane 1), ethanol (lane 2) or TNBS (lane 3) 7 days earlier. Position of NHE-1 is shown. Bar diagram showing (on the y-axis) increases in the NHE-1 protein levels (band area) in the crude membranes from rats that received TNBS (bar 2) 7 days earlier as compared with the PBS control (bar 0) or the ethanol control (bar 1) on the x-axis. Data are mean ± S.E.M. (n = 6, P < .03).

	Discussion

Top Abstract Introduction Materials & Methods Results Discussion References

Four NHE isozymes are known at present, among which NHE-1 is a ubiquitous isozyme. It is located on the basolateral side ofthe epithelial cells in the GI tract (Bianchini and Pouyssegur,1995; Noel and Pouyssegur, 1995). We demonstrate that the isoformsNHE-1 (present study), NHE-2, NHE-3 and NHE-4 mRNA (data not shown)are expressed in the colonic mucosa at varying levels. Our findingsshow increased levels of NHE-1 mRNA and protein in HAC-inducedcolitis. Physiologically, NHE induction may be important in maintainingthe pH_i of colonocytes acidified by HAC. It is relevant to mentionthat the colonocytes from patients with Crohn's disease show decreasedpH_i (Rowe and Bobar, 1995). However, at this point we do not knowwhether the pH_i of the colonocytes is decreased in the modelsof colitis used in the present study. Acidosis induces the NHE-1activity (L'Allemain et al., 1984). Whether pH_i is a primary ora secondary factor in the induction of NHE-1 remains to be known.Because other isoforms are also increased by colitis, we suggestthat acidosis may be a secondary phenomenon and that thereforeNHE-1 should contribute significantly to the pH_i, cell growthand tissue repair during IBD. This notion is further supportedby a similar increase in mRNA during TNBS-induced colitis. Thesefindings suggest that the induction of NHE-1 is independent ofthe way colitis is induced. NHE plays an important role in cellularinjury, hypertrophy and proliferation of smooth muscle cells andother cell types (Takewaki et al., 1995). It is relevant to mentionthat in intestinal inflammation, hyperplasia of smooth musclecells and epithelial cells has been reported (Blennerhassett etal., 1992, MacDonald, 1992). We believe that NHE-1 might be beneficialin the repair of tissue injury caused by the colitides. Althoughour mucosal scrapings contained predominantly epithelial cells,we also noticed a large infiltration of inflammatory cells inthe inflamed colon (data not shown). Therefore, changes in theNHE-1 do not reflect epithelial cells exclusively. The underlyingmechanism of the induction of mRNA may involve transcription activationand or stabilization of mRNA; this hypothesis requires furtherconfirmation. Both models were characterized by measuring theMPO activity, which was suppressed significantly by dexamethasone.We also examined histological changes, which included epithelialerosion, loss of crypts and infiltration of inflammatory cellsin lamina propria and muscularis mucosa (data not shown). Thesefindings, together with the induction of MPO, confirm the inductionof colitis by the colitides.

We employed RT-PCR to estimate the level of NHE-1 mRNA, using as internal control the alfa-1 isoform of the sodium pump (Khanand Collins, 1993), which was amplified under similar conditionsfrom each sample. Because its expression is decreased during colitis,it was considered suitable to prove the specificity of changes.For quantitation, the conditions were optimized in the linearrange of amplification, using different cycle numbers. The ratioNHE:internal control was used to indicate the level of NHE-1 mRNA.Elevation of NHE-1 mRNA does not reflect a general increase inthe poly A⁺ RNA content because 1) the level of internal control decreased,2) the difference in yield of total RNA between control and treatedrats was not significant and 3) the quality and quantity of theRNA samples used in RT-PCR were comparable as seen on the agarosegel. In addition, slot blot analysis yielded increases in theNHE-1 mRNA levels that were not significantly different from theRT-PCR data. In several studies, Northern blot analysis used forNHE-1 mRNA analysis (Bookstein et al., 1994; Cho et al., 1994)has shown one specific NHE-1 band. However, inconsistencies ofthe transfer step or poly A⁺ bias are difficult to address by Northern blot analysis. Therefore,we used slot blot analysis in the present study. Taken together,these findings suggest that the changes in the NHE-1 expressionare specific. PCR being supersensitive poses a problem of carry-over,or genomic contamination. This was addressed by amplifying RNAwithout RT, which failed to amplify the specific PCR fragment.In addition, the PCR fragment was characterized by restrictionanalysis and nucleotide sequencing. These findings rule out contaminationof the genomic DNA in the RNA samples, or carry-over. It was difficultto control the number of epithelial cells in the mucosal preparation,so changes shown here are normalized to the total cellular RNAbut not the number of cells.

Because it has been suggested that proinflammatory cytokines stimulate NHE in other systems (Benos et al., 1994), in the presentstudy we were interested in identifying the role of inflammationin the induction of NHE-mRNA. Therefore, we examined the effectof dexamethasone 3 days after HAC and 7 days after TNBS administration.In both models, the MPO activity was significantly suppressedby dexamethasone treatment, whereas the NHE-1 mRNA remained unchanged.We selected the condition of HAC for the following reasons. First,this time-point was in the linear range of MPO activity profile.Second, on days 1 and 2 after administration, the colon was badlydamaged. Whereas in the HAC- or TNBS-inflamed colon MPO activitywas suppressed significantly, the level of NHE isoforms remainedunaltered by dexamethsone treatment. Because dexamethsone inhibitsthe synthesis of cytokines, these findings suggest that the cytokinesmay be a secondary factor in the induction of NHE-1 during colitis.Dexamethasone acts through its interactions with the glucocorticoidresponsive element (GRE) module in a gene promoter and activatesthe NHE-3 isoform (Cho et al., 1994; Yun et al., 1993).

In conclusion, we demonstrate that the NHE-1 mRNA and protein are induced in both models of colitis, which suggests that NHE-1expression is independent of the nature of the colitide. Becausecolitis-induced NHE-2 and NHE-3 mRNA levels were not suppressedby dexamethasone treatment of colitis, pH_i and cytokines may bea secondary factor in the induction of NHE-1 mRNA. Increases inthe expression of NHE-1 should contribute to pH_i and to cell growthand repair during colitis and, therefore, may be beneficial. Theregulation of the expression of NHE-1 might involve pretranslationalsteps that do not seem to be regulated primarily by cytokinesor pH_i.

	Acknowledgments

The authors are grateful to Dr. E. B. Chang for his kind gift of the NHE-1 antibodies and to Ms. Nancy R. Thomas for her technicalhelp. I.K. acknowledges the financial support of the Kuwait UniversityGrant no. MB026.

	Footnotes

Accepted for publication January 16, 1998.

Received for publication August 19, 1997.

Send reprint requests to: Dr. Islam Khan, Department of Biochemistry, Faculty of Medicine, Kuwait University, P.O. Box 24923, Kuwait.

	Abbreviations

HAC, acetic acid; TNBS, trinitrobenzenesulfonic acid; NHE, sodium hydrogen exchanger; RT-PCR, reverse transcription-polymerase chain reaction; ECL, enhanced chemiluminescence light; PBS, phosphate-buffered saline; SSC, sodium chloride and sodium citrate; MPO, myeloperoxidase; IBD, inflammatory bowel disease; MOPS, 3-(N-morpholino)-propanesulfonic acid; pH_i, intracellular pH.

	References

Top Abstract Introduction Materials & Methods Results Discussion References

Allgayer H, Kruis W, Paumgartner G, Weibecke B, Brown L and Erdmann E (1988) Inverse relationship between colonic (Na⁺-K⁺)-ATPase activity and degree of mucosal inflammation in inflammatory bowel disease. Dig Dis Sci 33: 417-422[Medline].
Benos DJ, McPherson S, Hahn BH, Chaikin MA and Benveniste EN (1994) Cytokines and HIV envelope glycoprotein gp120 stimulate Na⁺/H⁺ exchange in astrocytes. J Biol Chem 269: 13811-13816[Abstract/Free Full Text].
Bianchini L and Pouyssegur J (1995) Na⁺/H⁺ exchangers: Structure, function and regulation, in Molecular Biology of the Kidney in Health and Disease. (Schlondorff D andBonventre J eds) Dekker, New York.
Blennerhassett MG, Vignjevic P, Vermillion DL and Collins SM (1992) Inflammation causes hyperplasia and hypertrophy in smooth muscle of rat small intestine. Am J Physiol 262: G1041-G1046[Abstract/Free Full Text].
Bookstein C, Depaoli AM, Xie Y, Niu P, Musch MW, Rao MC and Chang EB (1994) Na⁺/H⁺ exchangers, NHE-1 and NHE-3, of rat intestine. J Clin Invest 93: 106-113.
Bradley PP, Priebat DA, Christensen RD and Rothstein G (1982) Measurement of cutaneous inflammation: Estimation of neutrophil content with an enzyme marker. J Invest Dermatol 78: 206-209[Medline].
Chirgwin JM, Przybyla AE, Macdonald R and Rutter WJ (1979) Isolation of biologically active ribonucleic acid from sources enriched in ribonuclease. Biochemistry 18: 5294-5299[Medline].
Cho JH, Musch MW, Depaoli AM, Bookstein CM, Xie Y, Burant CF, Rao MC and Chang EB (1994) Glucocorticoids regulate Na⁺/H⁺ exchange expression and activity in region- and tissue-specific manner. Am J Physiol 267: C796-C803[Abstract/Free Full Text].
Collins JF, Honda T, Knobel S, Bulus NM, Conary J, Dubois R and Ghisham FK (1993) Molecular cloning, sequencing, tissue distribution and functional expression of a Na⁺/H⁺ exchanger (NHE-2). Proc Natl Acad Sci (USA) 90: 3938-3942[Abstract/Free Full Text].
Dias VC, Wallace JL and Parsons HG (1992) Modulation of phospholipid fatty acid leukotriene B₄ synthesis in the human intestinal cell (CaCo-2). Gut 333: 622-627.
Grossi L, Mchugh K and Collins SM (1993) On the specificity of altered muscle function in experimental colitis in rats. Gastroenterology 104: 1049-1056[Medline].
Innis MA, Gelfand DH, Sninsky J and White TJ (1990) PCR Protocol: A Guide to Methods and Application. Academic, New York.
Justinichi C, Gurbindo C, Hiscott J, Duhaime A and Seidman E (1992) Tumor necrosis factor (TNF-alfa) is an autocrine-paracrine growth factor for a rat intestinal crypt cell line IEC-6 (Abstract). Gastroenterology 102: A559.
Khan I and Al-Awadi FM (1997) Colonic muscle enhances the production of interleukin-1 $beta$ messenger RNA in experimental colitis. Gut 40: 307-312[Abstract/Free Full Text].
Khan I, Al-Awadi FM and Abul H (1996) Altered expression of the isoforms of Na⁺/H⁺ exchanger in experimental colitis. Gastroenterology 110: A337.
Khan I and Collins SM (1993) Altered expression of sodium pump isoforms in the inflamed intestine of Trichinella spiralis-infected rats. Am J Physiol 264: G1160-G1168[Abstract/Free Full Text].
Khan I, Tabb T, Garffield RE and Grover AK (1992) Polymerase chain reaction assay of mRNA using 28s rRNA as internal standard. Neurosci Lett 147: 114-117[Medline].
Laemmli UK (1970) Cleavage of structural proteins during the assembly of the head of bacteriophage T₄. Nature (Lond) 227: 680-685[Medline].
L'Allemain G, Paris S and Pouyssegur J (1984) Growth factor action and intracellular pH regulation in fibroblasts. Evidence for a major role of the Na⁺/H⁺ antiport. J Biol Chem 259: 5809-5815[Abstract/Free Full Text].
Levine SA, Montrose MH, Tse CM and Donowitz M (1993) Kinetics and regulation of three cloned mammalian Na⁺/H⁺ exchangers stably expressed in a fibroblast cell line. J Biol Chem 268: 25527-25535[Abstract/Free Full Text].
Macdonald TT (1992) Epithelial proliferation in response to gastrointestinal inflammation. Ann N Y Acad Sci 664: 201-209.
Maher MM, Gontarek JD, Bess RS, Donowitz M and Yeo CJ (1997) The Na⁺/H⁺ exchange isoform NHE3 regulates basal canine ileal Na⁺ absorption in vivo. Gastroenterology 112: 174-183[Medline].
McPherson BR and Pfeiffer CJ (1977) Experimental production of diffuse colitis in rats. Digestion 17: 135-150.
Morris GP, BEck PL, Herridge MS, Depew WT, Szewczuk MR and Wallace JL (1989) Hapten-induced model of chronic inflammation and ulceration in the rat colon. Gastroenterology 96: 795-803[Medline].
Noel J and Pouyssegur J (1995) Hormonal regulation, pharmacology, and membrane sorting of vertebrate Na⁺/H⁺ exchanger isoforms. Am J Physiol 268: C283-C296[Abstract/Free Full Text].
Orlowski J, Kandasamy RA and Shull GE (1992) Molecular cloning of putative members of the Na/H exchanger gene family. J Biol Chem 267: 9331-9339[Abstract/Free Full Text].
Rowe WA and Bobar SM (1995) Intracellular pH of colonocytes is altered in patients with Crohn's disease. Gastroenterology 108: A319.
Sambrook J, Fritsch EF and Maniatis T (1989) Molecular cloning: A Laboratory Manual, 2nd ed. Cold Spring Harbor, N.Y.: Cold Spring Harbor Laboratory Press.
Shallat S, Schmidt L, Reaka A, Rao D, Chang EB, Rao MC, Ramaswamy K and Layden TJ (1996) NHE-1 isoform of the N⁺/H⁺ antiporter is expressed in the rat and rabbit esophagus. Gastroenterology 109: 1421-1428[Medline].
Takewaki S, Kuro-o M, Hiroi Y, Yamazaki T, Noguchi T, Miyagishi A, Nakahara K., Aikawa M., Manabe I, Yazaki Y. and Nagai R (1995) Activation of Na⁺/H⁺ antiporter (NHE-1) gene expression during growth, hypertrophy and proliferation of the rabbit cardiovascular system. J Mol Cell Cardiol 27: 729-742[Medline].
Tse CM, Brant SR, Walker MS, Pouyssegur J and Donowitz M (1992) Cloning and sequencing of a rabbit cDNA encoding an intestinal and kidney-specific Na⁺/H⁺ exchanger (NHE-3). J Biol Chem 267: 9340-9346[Abstract/Free Full Text].
Tse CM, Levine SA, Yun CHC, Brant SR, Pouyssegur J, Montrose MH and Donowitz M (1993) Functional characteristics of a cloned epithelial Na⁺/H⁺ exchanger (NHE3): Resistance to amiloride and inhibition by protein kinase C. Proc Natl Acad Sci (USA) 90: 9110-9114[Abstract/Free Full Text].
Volker G, Andus T, Daig R, Aschenbrenner E, Scholmerich J and Falk W (1995) Regulation of interleukin-8 production in human colon epithelial cell line (HT-29). Gastroenterology 108: 653-661[Medline].
Wang Z, Orlowski J and Shull GE (1993) Primary structure and functional expression of a novel gastrointestinal isoform of the rat Na/H exchanger. J Biol Chem 268: 11925-11928[Abstract/Free Full Text].
Wild G and Murray D (1989) Changes in Na,K-ATPase, sodium ion, and glucose transport in the isolated enterocytes in an experimental model of malabsorption. Dig Dis Sci 34: 1739-1744[Medline].
Yun CH, Gurubhagavatulla S, Levine SA, Montgomery JL, Brant SR, Cohen ME, Cragoe EJ, Pouyssegur J, Tse CM and Donowitz M (1993) Glucocorticoid stimulation of ileal Na⁺ absorptive cell brush border Na⁺/H⁺ exchange and association with an increase in message for NHE-3, an epithelial Na⁺/H⁺ exchanger isoform. J Biol Chem 268: 206-2011[Abstract/Free Full Text].

This Article

	Abstract
	Full Text (PDF)
	Submit a response
	Alert me when this article is cited
	Alert me when eLetters are posted
	Alert me if a correction is posted
	Citation Map

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager

Citing Articles

	Citing Articles via Google Scholar

Google Scholar

	Articles by Khan, I.
	Articles by Abul, H.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Khan, I.
	Articles by Abul, H.