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APPETITE, OBESITY, DIGESTION, AND METABOLISM

Oxidative phosphorylation and its coupling to mitochondrial creatine and adenylate kinases in human gastric mucosa

¹Department of Pathophysiology, Centre of Molecular and Clinical Medicine, Faculty of Medicine, Department of Surgery, University of Tartu, Tartu, Estonia; ²Institute of Cell Biology, ETH Zürich, Zürich, Switzerland

Submitted 8 March 2006 ; accepted in final form 17 May 2006

	ABSTRACT

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Energy metabolism in gastrobiopsy specimens of the antral and corpus mucosa, treated with saponin to permeabilize the cells, was studied in patients with gastric diseases. The results show twice lower oxidative capacity in the antral mucosa than in the corpus mucosa and the relative deficiency of antral mitochondria in complex I. The mucosal cells expressed mitochondrial and cytosolic isoforms of creatine kinase and adenylate kinase (AK). Creatine (20 mM) and AMP (2 mM) markedly stimulated mitochondrial respiration in the presence of submaximal ADP or ATP concentrations, and creatine reduced apparent K_m for ADP in stimulation of respiration, which indicates the functional coupling of mitochondrial kinases to oxidative phosphorylation. Addition of exogenous cytochrome c increased ADP-dependent respiration, and the large-scale cytochrome c effect (20%) was associated with suppressed stimulation of respiration by creatine and AMP in the mucosal preparations. These results point to the impaired mitochondrial outer membrane, probably attributed to the pathogenic effects of Helicobacter pylori. Compared with the corpus mucosa, the antral mucosa exhibited greater sensitivity to such type of injury as the prevalence of the large-scale cytochrome c effect was twice higher among the latter specimens. Active chronic gastritis was associated with decreased respiratory capacity of the corpus mucosa but with its increase in the antral mucosa. In conclusion, human gastric mucosal cells express the mitochondrial and cytosolic isoforms of CK and AK participating in intracellular energy transfer systems. Gastric mucosa disease is associated with the altered functions of these systems and oxidative phosphorylation.

human stomach mucosa; corpus; antrum

There exists evidence that mitochondria may play an important role in development of gastric inflammation not only as being a source and target of the ROS (43) but also as the organelles specifically attacked by H. pylori. In cultured gastric cell lines the vacA cytotoxin of H. pylori directly impairs mitochondrial function seen as decreased rate of mitochondrial respiration, diminished membrane potential and ATP production (29), mitochondrial fragmentation (5), release of cytochrome c (34), and activation of apoptosis (16). Mitochondrial contribution may vary between the corpus and antral mucosa, because the former contains more mitochondria than the latter (35, 50), and H. pylori-linked inflammation is associated with higher activation of SOD because of upregulation of its mitochondrial isoform in the antrum but not in the corpus (8, 14, 18, 19). Yet it is unclear whether these diversities affect regulation and intracellular organization of energy metabolism in the mucosa. In many cells with high-energy requirements (skeletal muscle, cardiac muscle, brain, retina, and spermatozoa), mitochondria and ATPases are linked to each other by specialized phosphotransfer systems mediated by different creatine kinase (CK) and adenylate kinase (AK) isoforms. These systems carry out three consequent processes: 1) functional coupling between mitochondrial CK (MtCK) or AK2 isoforms with adenine nucleotide translocase (ANT); 2) transfer of the energy-rich phosphoryl group via cytosolic muscle-type (MM)-, heteromeric (MB)- or brain-type (BB)-CK (depending on the type of tissue) or AK1 isoforms; and 3) regeneration of ATP in the vicinity of ATPases because of the functional coupling of MM- or BB-CK or AK1 isoforms to ATPases (13, 47). Such an organization of intracellular energy metabolism enables precise matching between mitochondrial ATP synthesis and its consumption (13, 46, 47). Marked CK and AK activities have been detected in cultured gastric mucosal cells (21, 44, 55). In parietal cells BB-CK is strongly expressed (55, 63) and colocalizes and functionally couples to H⁺-K⁺-ATPase to effectively provide ATP for proton pumping (55). On the other hand, exchange between adenine nucleotides mediated by AK is markedly activated in the conditions of generation of ATP by mitochondria (44). Although these data point to the possible participation of CK and AK isoforms in the energy transfer systems in human gastric mucosal cells, the evidence confirming this is still lacking.

This study was undertaken to comparatively characterize the energy metabolism in biopsy specimens from the antral and corpus mucosa of the patients undergoing gastric endoscopy for diagnostic purposes. The function of the respiratory chain and the status of oxidative phosphorylation, the activities of AK and CK, and the expression of their mitochondrial and cytosolic isoforms, as well as the coupling of mitochondrial kinases to oxidative phosphorylation were assessed in gastrobiopsy specimens after permeabilization of the cells with saponin. This approach enables characterization of the mitochondrial function in situ, i.e., in a natural interaction of mitochondria with kinases, ATPases, and other cell structures (48, 53). We showed that the antral mucosa exhibits twice lower respiratory capacity and a relative deficiency in complex I of the respiratory chain compared with the corpus mucosa. These changes are probably attributable to normal tissue-specific differences. Both antral and corpus mucosal cells express mitochondrial isoforms of AK and CK, functionally coupled to mitochondrial ATP production, which supports the hypothesis that mucosal cells possess a system of intracellular energy transfer. Also, we provided evidence that disorders of the gastric mucosa affect the processes of oxidative phosphorylation and energy transfer differently in the antrum and in the corpus.

	METHODS

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Subjects and Gastric Mucosa Sampling

Gastric biopsies were carried out in accordance with the European Communities Council Directive 86/609/EEC and with the Declaration of Helsinki (64). Written informed consent was obtained from all patients, and the Tartu University Ethics Committee approved the study.

Forty consecutive patients (23 male and 17 female, aged 60 ± 2.3 and 64 ± 3.0 years, respectively) from southern Estonia who underwent upper gastrointestinal endoscopy due to epigastric complaints were included in this study. At endoscopy, different lesions were detected, such as esophagitis, hiatus hernia, gastric mucosal erosions, gastric or duodenal ulcer, duodenitis, and gastric cancer. Most of the patients (71%) were histologically H. pylori positive, which corresponds to the serological finding that 80% of the inhabitants of Estonia are carriers of that bacterium. Its virulence is highly expressed as 87% of patients with the different gastric diseases presented the cagA gene that correlated strongly with the vacA signal sequence type s1a (3). None of the subjects had received nonsteroidal anti-inflammatory drugs, H⁺-pump inhibitors, or antibiotics to cure the illness. Mucosal biopsies were taken from the antrum (2 cm above the pylorus from the anterior and posterior walls of the stomach) and from the anterior wall and posterior wall of the medial part of the corpus. In the patients with gastric cancer, the specimens were taken from the apparently normal mucosal region apart from the tumor tissue. One part of each biopsy specimen was used to determine the histology of the gastric mucosa and the presence of H. pylori, for which these specimens were fixed overnight in neutral buffered formalin and embedded in paraffin. Tissue sections were stained for morphological and H. pylori examination by the hematoxylin and eosin and modified Giemsa methods. The presence and severity of chronic gastritis, activity of gastritis, atrophy, and intestinal metaplasia were graded according to the Sidney system from 0 (no changes) through 1 (mild) and 2 (moderate) to 3 (severe changes) (12). Infiltration of lymphocytes was taken to indicate the chronic status of inflammation, and abundant presence of mononuclear cells was taken to mark an active chronic process. The amount of H. pylori in the mucosa was estimated semiquantitatively by microscopic counting as described earlier (42). Another part of the antral and corpus mucosa specimens was transferred into the RNA-Later reagent (Qiagen) for RNA extraction, and the third part was placed in the ice-cold solution A containing (in mM): 2.77 CaK₂EGTA, 7.23 K₂EGTA, 6.56 MgCl₂, 0.5 DTT, 50 K-Mes, 20 imidazole, 20 taurine, 5.3 Na₂ATP, 15 phosphocreatine, 7.1 pH, and was used for permeabilization of the cells. Because of the limited sample availability, the number of specimens studied in different experiments varied as shown in the figure legends.

Preparation of Permeabilized Mucosal Tissue

The mucosal tissue samples were cut into 1 x 1.5-mm pieces in the ice-cold solution A. With the use of thin needles, the tissue pieces were gently stretched in all directions to mechanically separate the cells from each other. The tissue was then transferred into vessels with ice-cold solution A containing 50 µg/ml saponin and incubated at mild stirring for 30 min for permeabilization of the plasmalemma due to removal of cholesterol from the cell membrane by saponin. The indicated conditions were found to be optimal for maintaining mitochondrial function inside the permeabilized cells. The permeabilized mucosal tissues were then washed three times in solution B containing (in mM): 2.77 CaK₂EGTA, 7.23 K₂EGTA, 1.38 MgCl₂, 0.5 DTT, 100 K-Mes, 20 imidazole, 20 taurine, 3 K₂HPO₄, 10 glutamate and 2 malate, and 5 mg/ml bovine serum albumin, 7.1 pH at 25°C to remove all metabolites. The extent of permeabilization was monitored by the leakage of lactate dehydrogenase (LDH), a 145-kDa cytosolic protein. The cells lost about 60-70% of LDH during saponin treatment, which corresponds to the data obtained from the study of digitonin-permeabilized rabbit gastric glands (1).

Analysis of Oxidative Phosphorylation and Its Coupling to MtCK

The saponin-treated tissues were incubated in solution B containing (mM): 2.77 CaK₂EGTA, 7.23 K₂EGTA, 1.38 MgCl₂, 0.5 DTT, 100 K-Mes, 20 imidazole, 20 taurine, 3 K₂HPO₄, 10 glutamate, and 2 malate, and 5 mg/ml bovine serum albumin, pH 7.1 at 25°C, in a chamber (volume 1.5-2.5 ml) of oxygraph (Rank Brothers, England or Oroboros, Paar KG, Austria), equipped with the Clark electrode, assuming the solubility of oxygen in the medium to be 215 nM O₂/ml (32). After the registration of basal respiration rate (V₀) in nonphosphorylating conditions in the presence of 10 mM glutamate and 2 mM malate, 2 mM ADP was added to monitor the maximum rate of NADH-linked ADP-dependent respiration (V_Glut), followed by successive additions of 10 µM rotenone to inhibit the complex I, 10 mM succinate to activate FADH₂-linked ADP-dependent respiration (V_Succ), 0.1 mM atractyloside to assess respiratory control by ANT, 10 µM antimycin A to inhibit the electron flow from the complex II to cytochrome c, 0.5 mM N,N,N,'N'-tetramethyl-p-phenylenediamine (TMPD) with 2 mM ascorbate to activate cytochrome c oxidase (COX), and 5 mM NaN₃ to quantify COX activity (V_COX) as the NaN₃-sensitive portion of respiration. Antimycin-sensitive respiration in the presence of atractyloside was considered to measure the respiration related to proton leak. The coupling between oxidative phosphorylation and MtCK was estimated using two protocols.

Protocol 1. After the registration of V₀ in nonphosphorylating mitochondria in solution B with glutamate plus malate, 50 µM ATP was added to produce a minimum amount of endogenous ADP to stimulate mitochondria. AMP (2 mM) was then added to activate the coupled reaction of AK2 with ANT followed by addition of 0.2 mM diadenosine pentaphosphate (AP₅A) to inhibit AK (52). To assess the strength of the functional coupling independently of mitochondrial content in individual mucosal preparations, activation of respiration by AMP was normalized for the respiratory rate registered before the addition of AMP, thus producing the relative index (I_AK): [I_AK = (V_AMP – V_ATP)/V_ATP]. After AP₅A, 20 mM creatine (Cr) was added from solid to induce the coupling between MtCK and ANT, the efficiency of which was measured as CK index (I_CK): [I_CK = (V_Cr – V_AP5A)/V_AP5A]. Thereafter, 2 mM ADP was added for maximum activation of respiration (V_ADP) and 0.1 mM atractyloside was added to monitor control by ANT over oxidative phosphorylation. The maximum capacity of the respiratory chain was estimated in the presence of 2 µM carbonyl cyanide p-trifluoromethoxyphenylhydrazone (FCCP) (V_FCCP). In the same protocol, the intactness of mitochondrial outer membrane (MOM) was controlled by the addition of 8 µM cytochrome c (48, 52).

Protocol 2. The O₂ vs. [ADP] relationships were examined in solution B supplemented with 10 mM glutamate, 2 mM malate, 4 U/ml hexokinase, and 11 mM glucose in the presence and absence of 20 mM creatine, and the corresponding apparent K_m and V_max values were calculated.

Determination of the Activity of Total ATPase, AK, and CK in Permeabilized Gastric Mucosa

The permeabilized mucosal specimens were incubated in a spectrophotometric cuvette in stirring conditions in the medium containing (in mM): 20 Tris·HCl (pH 8.0, 30°C), 15 KCl, 0.3 DTT, 0.24 NADH, 0.8 phosphoenolpyruvate (PEP), and 6 IU/ml pyruvate kinase (PK) and 3 IU/ml LDH. To register total ATPase activity, 1 mM of ATP together with 0.8 mM MgCl₂ was added, and the decrease in NADH concentration was measured at 340 nm by using PerkinElmer Lambda 900 spectrophotometer. AMP (1.3 mM) was then added to determine AK activity followed by the addition of 20 mM creatine to measure CK activity. Care was taken that the measured reactions occurred linearly in time and that the coupled enzyme systems were not limiting overall reaction rate.

Determination of the LDH Activity

Tissue samples were frozen in liquid nitrogen and homogenized in 300 µl of phosphate buffer (50 mM, pH 7.3) by Ultra-Turrax homogenizer (Janke and Kunkel, IKA Labortechnik, Germany) at a speed of 13,500 rpm/min for 30 s at +4°C. Then Triton X-100 was added (1% final concentration), and the homogenate was incubated for 1 h on ice. The LDH activity was measured spectrophotometrically at 340 nm in the medium containing aliquot, 0.265 mM NADH, and 50 mM phosphate buffer (pH 7.3 at 25°C). Reaction was initiated with 3 mM sodium pyruvate.

RNA Preparation

Total RNA from the mucosal biopsies was prepared at room temperature using the Qiagen RNeasy Protect Mini Kit, according to the manufacturer's protocol. Approximately 25 mg of mucosal tissue from the antrum and corpus of the same patient was immediately placed into the RNAlater RNA stabilization reagent for tissue transportation and storage until homogenization and lysis. Disruption and homogenization of the tissue were carried out in lysis buffer (supplied in the kit) by an Ultra-Turrax homogenizator (Janke and Kunkel, IKA Labortechnik) at a speed of 8,000 rpm/min for 30 s. Ethanol (70%) was then added to lysate, and the samples were applied to the RNeasy column (Qiagen). The contaminants (e.g., lysis buffer components) were removed by one wash spin at 8,000 g with the buffer RW1 and by two wash spins at 8,000 g with the washing buffer RPE (both supplied in the kit). Finally, membrane-bound total RNA was eluted in 30 µl RNAse-free water. RNA concentration in elute was determined by measuring the absorbance in 10 mM Tris·HCl, pH 7.5 at 260 nm. The RNA isolated appeared to be pure since its 260/280 absorbance ratio varied between 1.9 and 2.0. The integrity of RNA was examined by electrophoresis in an ethidium bromide stained 0.8% agarose gel (38), which revealed two characteristic ribosomal 28S and 18S bands, without any evidence of RNA degradation (Fig. 2).

View larger version (7K): [in this window] [in a new window]   Fig. 1. Total activities of ATPases, adenylate kinase (AK), and creatine kinase (CK) in the human permeabilized gastric mucosa from the antrum (open bars, n = 18) and corpus (filled bars, n = 18). Here and elsewhere, the means ± SE and the number of specimens (n) studied are given. *P < 0.05, **P < 0.01 vs. corpus. ww, wet weight.

View larger version (50K): [in this window] [in a new window]   Fig. 2. A: ribosomal bands 28S and 18S of total RNA purified from the corpus and antral mucosa of a patient with peptic ulcer. B: PCR products of two AK genes (AK1, AK2) and two CK genes (CKB, CKMT1) amplified from the corpus and antral mucosa of the same patient. A SYBR Green I stained 1.7% agarose gel with proposed amplicons is shown. The left trace (M) indicates DNA size marker (100 bp; Generuler, Fermentas, Lithuania). Gene symbols are given according to GenBank, i.e., the National Institutes of Health, U.S. Genetic Sequence Database of the National Center of Biotechnology Information.

One microgram of total RNA was used for reverse transcription into single-strand cDNA using SuperScript II reverse transcriptase (Invitrogen). One microliter oligo(dT) at a concentration of 500 µg/ml and 1 µl 10 mM dNTP mix were added to the aforementioned amount of RNA and heated to 65°C for 5 min; thereafter, the mix was quickly chilled on ice. Final reaction volume contained (in mM) 0.5 dNTP, 10 DTT, 50 Tris·HCl (pH 8.3), 75 KCl, and 3 MgCl₂, and 2 U/µl RNAse inhibitor (Fermentas). Reverse transcription was performed at 42°C for 50 min. After that the reaction was inactivated by heating at 70°C for 15 min. The obtained transcripts were used for polymerase chain reaction (PCR).

PCR Reactions

The forward and reverse oligonucleotide primer pairs (Table 1), to match the sequences of human AK1, AK2, brain-type CK (B-CK), and uMtCK, were designed by the Primer Express software (Applied Biosystems). PCR amplification was performed using the QuantiTect SYBR Green PCR Kit (Qiagen) with the ABI PRISM 7000 Sequence Detection System (Applied Biosystems). The thermal profile for RT-PCR comprised initially 15 min at 94°C to activate HotStarTaq DNA. This was followed by 35 cycles of denaturation at 94°C for 15 s, annealing at 55°C for 30 s, and extension at 72°C for 30-s steps. After the 35th cycle, the amplified cDNAs were separated in a 1.7% agarose gel to verify amplicons by size.

Thirty-five micrograms of total protein in homogenates was separated by standard 12% SDS-PAGE and electrotransferred by semidry blotting (Hoefel Pharmacia Biotech, San Francisco, CA) on a nitrocellulose membrane (Shleicher and Schüell, Dassel, Germany), according to the manufacturer's instructions. The membranes were blocked with 4% fat-free milk powder in T-TBS (20 mM Tris·HCl pH 7.5, 150 mM NaCl, 0.05% Tween 20) overnight at 4°C, incubated for 15 min at room temperature and washed for 4 x 5 min with T-TBS. The membranes were then incubated for 1 h with uMtCK rabbit immunesera (1:2,000 dilution in a blocking buffer) or with affinity-purifed chicken anti-B-CK IgY (1:500 dilution in a blocking buffer) at room temperature (51). For detecting AKs, the membranes were incubated for 1 h at room temperature with rabbit polyclonal antibodies against AK1 (H-90; Santa Cruz Biotechnology, Santa Cruz, CA) or AK2 (H-65; Santa Cruz Biotechnology) (dilution 1:500 in a blocking buffer), washed for 4 x 5 min in T-TBS and incubated for 1 h with the peroxidase-coupled secondary antibody, either goat anti-rabbit IgG (Nordic, Lausanne, Switzerland) (1:1,000 dilution in a blocking buffer) or rabbit anti-chicken IgY (Jackson ImmunoResearch, West Grove, PA) (1:3,000 dilution in a blocking buffer), and finally washed for 4 x 5 min with T-TBS. The blots were developed with the enhanced chemiluminescence substrate (Amersham, Buckinghamshire, UK) and exposed to an X-ray film.

Statistical Analysis

The means ± SE are presented. Differences between the groups were evaluated using Student's t-test.

	RESULTS

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Function of Oxidative Phosphorylation in Gastric Mucosa

Table 2 summarizes the analysis of the function of the respiratory chain in the permeabilized mucosal specimens from the antrum and corpus. For the antrum mucosa, the mean values of all respiratory rate indices (V₀, V_Glut, V_Succ, V_Atr, V_COX, and V_FCCP) were lower than for their corpus counterparts (by a factor of 1.6, 2.3, 1.7, 2.1, 2.1, and 1.8, respectively), which refers to less tissue content of mitochondria in antral mucosa. When the ratios of respiration rates with different substrates, independent of individual variation of mitochondrial content, were compared in the same mucosal specimen, different functional properties of mitochondria in antrum and corpus became evident. In corpus, the V_Glut-to-V_Succ ratio was 1.38, comparable to that in other tissues, such as muscle or heart in the healthy state (17, 52), and the V_Glut-to-V_COX ratio exceeded the V_Succ-to-V_COX ratio. Thus complex I-dependent respiration was higher than complex II-dependent respiration, which implies limitation of the electron flow at the level of complex II. Compared with the V_Glut-to-V_Succ ratio in the corpus, this parameter was reduced in the antral mucosa. Presumably, this change resulted from a combination of decreased complex I-dependent respiration and increased complex II-dependent respiration, as suggested by the tendencies to reciprocal alterations in V_Glut-to-V_COX and V_Succ-to-V_COX ratios. Compared with the corpus mucosa, the antral mucosa exhibited lower respiration control index (RCI)_Glut but higher RCI_Succ, this difference being attributable to a larger deficit in V_Glut than in V_Succ, to a smaller deficit in V₀ than in V_Atr, and to a smaller proton leak.

The activities of total tissue ATPase and CK in the corpus mucosa exceeded those in the antrum mucosa, while no difference between these tissues was observed in total AK activity (Fig. 1). Figure 2 shows that the antral and corpus mucosa expressed mRNA encoding mitochondrial (AK2 and ubiquitous CKMT1) and cytosolic (AK1 and CKB) isoforms of AK and CK, respectively. The expression of CKM originating from the microvessels and the muscularis mucosae layer was negligible (not shown), which suggests that the expression signals for AK and CK emerged chiefly from the epithelial cells. A Western blot analysis of the tissue homogenates confirmed the presence of the B-CK, uMtCK, AK1, and mitochondrial AK2 proteins (Fig. 3). The presence of mitochondrial and cytosolic isoforms of CK and AK points to the existence of intracellular energy transfer systems linking mitochondria to ATPase. The presence of the functional coupling between mitochondrial kinases and ANT, a key stage in these systems, was tested by means of two previously validated protocols (52). In one of them (Fig. 4) the permeabilized mucosal cells were incubated with 50 µM ATP, which led to a minimum stimulation of respiration because of the limited amounts of ADP that the ATPases could produce. Addition of 2 mM AMP strongly stimulated respiration as it triggered the functional coupling of mitochondrial AK2 to ANT, thereby increasing the local [ADP] near ANT. Participation of AK in this process was confirmed by the effect of the AK inhibitor AP₅A: suppression of respiration down to the levels before AMP addition. Inclusion of 20 mM creatine reactivated respiration, because now MtCK, coupled to ANT, provided a local activator, ADP. Stimulation of respiration with AMP was stronger than stimulation with creatine because each cycle of AK2 reaction coupled to ANT produced two times more ADP compared with MtCK reaction (52). The I_AK, an index independent of the tissue mitochondrial content, was smaller for the antrum (0.517 ± 0.038, P < 0.05, n = 27) than for the corpus (0.651 ± 0.050, n = 27). This change may indicate a less tight coupling between AK2 and ANT and/or less active AK2 in the antrum mucosa. Regarding I_CK, a similar tendency was observed, although without statistical significance (0.372 ± 0.056, n = 26, and 0.504 ± 0.090, n = 26, in the antrum and corpus, respectively).

View larger version (21K): [in this window] [in a new window]   Fig. 3. Immunoblots tested with polyclonal rabbit antibodies against AK1, AK2, ubiquitous MtCK (uMtCK), and affinity-purified chicken IgY antibodies against B-CK. Homogenized mucosal tissue containing 35 µg total protein from the antrum or corpus was used. To verify B-CK and uMtCK, recombinant human proteins (1 µg) expressed in Escherichia coli were applied as positive controls. For AKs, 35 µg of protein from the cytosolic and mitochondrial (37a) fractions of the rat heart were used as positive controls for AK1 and AK2, respectively. To compare the size of the proteins, the position of the marker proteins with given molecular mass is shown on the right side of each panel.

View larger version (8K): [in this window] [in a new window]   Fig. 4. Original recording of a respirometric investigation of the coupling of AK and CK to oxidative phosphorylation in a permeabilized mucosal specimen from the gastric corpus. O2 was measured in the presence of 10 mM malate and 2 mM glutamate as respiratory substrates. Additions: tissue, permeabilized mucosal tissue 2-5 mg ww; 50 µM ATP; 2 mM AMP; 0.2 mM diadenosine pentaphosphate (AP5A); 20 mM creatine (Cr); 2 mM ADP; 0.1 mM ATR; 2 µM FCCP; and 8 µM cytochrome c (Cyt c). ATR, atractyloside.

View larger version (15K): [in this window] [in a new window]   Fig. 5. The effect of 20 mM creatine on the kinetics of regulation of respiration by exogenous ADP. A: O2 vs. concentration of ADP {[ADP]) relationships in double-reciprocal coordinates (+Cr, with creatine, –Cr, without creatine). B: apparent Km. C: Vmax in permeabilized gastric mucosa. B and C: filled bars, +Cr; open bars, –Cr; n = 6 for each group compared. *P < 0.05, **P < 0.01 compared with assessment –Cr. +++P < 0.001 vs. corpus.

View larger version (10K): [in this window] [in a new window]   Fig. 6. Relationships between the extent of cytochrome c effect on ADP-stimulated respiration (%) and coupling of mitochondrial kinases expressed as CK index (ICK; A) and AK index (IAK; B) in permeabilized gastric mucosa. Open bars, n = 33, A and B; filled bars, n = 19 (A) and n = 21 (B). *P < 0.05 vs. preparations with the cytochrome c effect <20%.

View larger version (10K): [in this window] [in a new window]   Fig. 7. The effect of active chronic gastritis (filled bars, n = 10 and 9 for antrum and corpus group, respectively) on respiratory parameters compared with absence of active process (open bars, n = 17 and 18 for antrum and corpus group, respectively) in permeabilized mucosa. *P < 0.05, **P < 0.01 vs. control without active process. V0, basal respiration rate.

	DISCUSSION

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Mucosal oxidative capacity was far higher in the corpus than in the antrum, in accordance with the larger content of mitochondria in the corpus mucosa (35, 50). The prominent oxidative capacity of the corpus mucosa relates to massive acid generation by parietal cells for which the mitochondria account for 25-45% of cell volume (24, 67). The tissue-specific differences were related not only to the amount of mitochondria but also to their functional properties, as indicated by decreased V_Glut-to-V_Succ ratio, RCI_Glut, and proton leak, but also by increased RCI_Succ in the antrum compared with corpus. Because a reduced V_Glut-to-V_Succ ratio is considered to be a reliable index of respiratory chain deficiency at the level of the complex I as observed in gene-modified animals and in human muscle disease (17, 45, 62), the low V_Glut-to-V_Succ ratio can be taken to indicate the impaired complex I function resulting from the pathogenic effects of H. pylori. However, the diminished complex I activity is also seen in the mitochondria of healthy rabbit antral mucosa, as indicated by a twice lower RCI, because of reduced state 3 respiration with glutamate compared with the corpus mitochondria (35). Besides, the normal antral mucosa contains more GHS than its corpus counterpart, which renders the former less susceptible to free radical damage during ischemia-reperfusion (58). Thus it could be speculated that the relative complex I deficiency is a normal property of the antral mitochondria, in which the increased antioxidative capacity serves to neutralize the excess ROS produced during hampered electron flow through the inadequate complex I, similarly to the processes taking place in many types of cells in response to the failure of complex I (43). Having considered these mechanisms, the role of variations in the complex II function as a reason for altered V_Glut-to-V_Succ ratio should not be overlooked. For example, fumarase deficiency is associated with suppressed succinate-dependent respiration (11), whereas atrial fibrillation is characterized by its increase (52), without changes in NADH-linked respiration. Our findings that the V_Succ-to-V_COX ratio tended to increase and the V_Succ was relatively less reduced than V_Glut in the antrum compared with corpus imply that the electron transfer from succinate to oxygen was less limited in the mitochondria of antral mucosa. Hence, this change could also contribute to the relative deficit in complex I in that type of mucosa. However, further studies, aimed at direct assessment of the enzyme activities of different respiratory chain complexes in these two types of gastric mucosa, are required to validate that assumption.

For the first time, this study demonstrates different responses of mitochondria to active chronic inflammation in the antral and corpus mucosa, as oxidative phosphorylation (e.g., measured as V_ADP) was suppressed in the corpus but was upregulated in the antrum (Fig. 7). These changes are surprising because active chronic gastritis and associated oxidative stress induced by H. pylori are always more pronounced in the antral than in the corpus mucosa (6, 15, 40), which would predict a more severe injury of antral mitochondria. Yet this apparent controversy can be explained by a tissue type-specific control of the cellular bioenergetic processes by this bacterium. First, H. pylori induces expression of mitochondrial MnSOD exclusively in the antral mucosa (8, 14, 18, 19), which might enhance its capacity to eliminate ROS, in addition to that afforded by intrinsically excessive GSH. Second, suppression of mitochondrial respiration in the corpus mucosa might result from inhibition of acid production. This assumption relies upon the findings that IL-1 and the TNF-, the two major cytokines mediating H. pylori effects, strongly inhibit acid secretion in cultured parietal cells (7) and that treatment of patients with omeprazole, a H⁺-K⁺-ATPase inhibitor, simultaneously downregulates mitochondrial activity (23). Finally, in our experiments, the H. pylori-linked inflammation was associated with concerted changes in V_ADP, V₀, and V_FCCP, without variations in RCI. Thus it seems that H. pylori effects were not related to regulation of mitochondrial function but to changes in tissue mitochondrial content that decreased in the corpus but increased in the antrum. In principle, these inverse changes could result from the differently altered balance between the antiapoptotic and apoptotic pathways in the corpus and antral mucosa. H. pylori promotes apoptosis mainly through the mitochondrial route by triggering cytochrome c release (16, 34) via translocation of Bax (5, 34) and/or the NH₂-terminal 34-kDa fragment of H. pylori vacA cytotoxin into the mitochondria (16) in association with depolarized mitochondrial membranes, depressed cellular respiration and ATP content, and mitochondrial fragmentation (5, 29). Among major pathogenic factors inducing these changes is ammonia, a product of strong urease activity of H. pylori (31, 56, 60, 61). Therefore, suppressed respiration (Fig. 7) in the gastric corpus mucosa can be related to apoptotic changes in the mitochondria. On the other hand, H. pylori exerts a powerful antiapoptotic influence through many ways, such as activation of the cellular inhibitor of the apoptosis 2 gene (66), epithelial cell-cycle arrest (54), and upregulation of cyclooxygenase-2 (COX-2) in epithelial, mononuclear, and parietal cells (15, 36, 59). The products of COX-2 (15d-PGJ₂ and PGA₁) directly inhibit NF-B-mediated apoptotic pathways via activating the peroxisome proliferator-activated receptor- (PPAR) (20, 41), whereas PPAR accelerates biosynthesis of mitochondria, thus increasing the tissue's oxidative capacity (9, 33). It is known that H. pylori upregulates COX-2 in the antral mucosa to a greater extent than in the corpus mucosa (15). Hence, activation of PPAR should also be more pronounced in the antral mucosa, which could account for the augmented respiration in this tissue registered by us (Fig. 7). Besides these mechanisms, host response to H. pylori involves increased gastrin production by mucosal G-cells, which in turn stimulates gastric epithelial cell proliferation (41). Thus it cannot be excluded that at least a fraction of increased oxidative capacity in the antrum stemmed from proliferation of G-cells.

Coupling of Mitochondrial Kinases to Oxidative Phosphorylation in Gastric Mucosa

Observations that short-term inhibition of proton pumps (H⁺-K⁺-ATPase) with omeprazole or ranitidine suppresses mitochondrial activity in the body of the human stomach (23), that blockade of mitochondrial processes abolishes the H⁺-pumping activity of the gastric glands (44), and that alterations in the secretory activity of parietal cells occur together with changes in mitochondrial morphology (25, 57), collectively imply that gastric mucosal cells must possess intracellular mechanisms enabling exact regulation of mitochondrial ATP production in accordance with altered ATP utilization in secretory processes.

In other types of cells, e.g., cardiomyocytes, these mechanisms are well characterized, and there exists consensus on the issue that mitochondria and ATPases communicate with each other via different isoforms of CK and AK coupled to ANT in mitochondria and to ATP-consuming processes at different intracellular sites (13, 46, 47). That CK is involved in these mechanisms in gastric mucosal cells was first demonstrated by Sistermans et al. (55), who showed a functional coupling between BB-CK and H⁺-K⁺-ATPase in parietal cells. Here we report that human gastric mucosal cells express not only BB-CK, but also uMtCK, which is functionally coupled to oxidative phosphorylation. To confirm this, one set of experiments demonstrated stimulation of respiration with creatine in the presence of minute concentrations of ATP (50 µM) (Fig. 4). Here, two principally different mechanisms can account for the creatine effect. First, creatine added to the medium, which represents cytoplasm in permeabilized cells, in the presence of ATP may activate cytosolic CK and the CK bound to endoplasmic reticulum and mitochondria, which increases stationary [ADP] in the cytoplasm/medium. The latter stimulates oxidative phosphorylation after being diffused through MOM and transported into the matrix. This mechanism described (Model I) assumes a fast equilibrium between ADP concentrations in the intermembrane space, cytosol, and medium to take place because of simultaneous action of cytosolic CK, AK, and ATPases. Alternatively, creatine could stimulate local production of ADP near ANT by MtCK at the expense of mitochondrially produced ATP. This mechanism (Model II), known as the functional coupling between ANT and MtCK, allows establishment of higher local concentrations of ADP in the microcompartment between MtCK and ANT than in the surrounding mitochondria cytoplasm (47).

To discriminate between these two models, the kinetics of regulation of mitochondrial respiration by ADP was analyzed from [ADP] vs. O₂ relationships in the presence of excess amounts of hexokinase and glucose. This system completely utilizes mitochondrial ATP once it reaches the cytosolic compartment to become available for hexokinase and allows clamping of cytosolic [ADP] at desired levels in experimental settings (Fig. 5). It was found that the apparent K_m value for ADP in regulation of respiration was 100 µM in both the antral and corpus mucosa, which is far higher than its value for the same process in isolated mitochondria (10-20 µM) (32). The concerns that the low apparent affinity of mitochondria to exogenous ADP in mucosal preparations is an artifact (resulting from incomplete permeabilization of cells or large diffusion distances within the bulk multicellular tissue) can be dispelled for several reasons. First, stimulation of respiration by cytochrome c (Figs. 4 and 6) directly demonstrates effective penetration of much larger molecules than ADP into the cell interior, thus indicating effective permeabilization. Second, glutamate-dependent respiration with exogenous ADP yielded a RCI value (2-3; Table 2) similar to that for mitochondria in homogenized mucosal preparations (50). Presence of intact (impermeabilized) cells in the medium would have resulted in RCI values lower than that for mucosal homogenates, due to the high rate of cellular respiration supported by endogenous ADP, which was not the case, however. Third, the straight-line double reciprocal relationships between the rates of respiration and [ADP] (Fig. 5) exclude existence of different populations of mitochondria with variable kinetic properties (e.g., mitochondria in permeabilized cells and intact cells, and mitochondria extracted from cells). Finally, high apparent K_m for ADP in regulation of respiration in oxidative muscle cells, permeabilized in the same manner as mucosal cells in this study, has been shown not to be proportional to cellular diffusion distances (i.e., cell dimensions), but related to organization of mitochondria and ATPases into compartmentalized functional complexes (53). Thus low apparent affinity of mitochondria to exogenous ADP registered in saponin-permeabilized mucosal cells likely stems from a specific structural and functional organization of their energy metabolism.

Further support for this assumption derives from the observation that creatine (20 mM) significantly activated respiration at low [ADP] thus giving rise to increased apparent affinity of mitochondria to exogenous ADP (Fig. 5, A and B). Considering the presence of hexokinase in activities significantly exceeding the total cellular ATP-consuming capacity [the sum of the activities of ATPases and forward CK (Fig. 1)], it is highly unlikely that extra ADP to stimulate respiration originated from the MM-CK reaction activated by creatine in the cytoplasmic bulk phase. Hence, it must have been the ATP pool inside the mitochondria (in the intermembrane space), inaccessible to hexokinase, that was converted to ADP by MtCK reaction in the presence of creatine to stimulate respiration. Because a local [ADP] near ANT builds up above corresponding submaximal [ADP] in the medium/cytoplasm in this process, the [ADP] vs. O₂ relationship changed toward diminished apparent K_m compared with its value without creatine (Fig. 5). This type of creatine effect on mitochondrial respiration is characteristic of the functional coupling between ANT and MtCK [Model II described above (47)]. These findings in combination with earlier results (55) allow us now to envisage the entire system of CK-phosphotransfer comprising all three necessary stages: 1) synthesis of PCr in mitochondria, 2) transfer of energy-rich phosphoryl groups from PCr via cytosolic BB-CK, and 3) regeneration of ATP in the vicinity of ATPases because of the coupling of BB-CK to ATPases in mucosal cells. Expression of mitochondrial (AK2) and cytosolic (AK1) isoforms and the coupling of mitochondrial ATP production to AK2 (Fig. 4) strongly suggest the presence of a functional AK-phosphotransfer network as well.

We found that mitochondria in gastric mucosa specimens exhibited leaky MOM, and the larger permeability of MOM was associated with decreased I_CK and I_AK (Fig. 6). The simplest explanation for these findings might be that the mitochondria degraded and lost their cytochrome c and kinases due to mechanical sample damage imposed during skinning procedure and the following oxygraphy. However, some lines of evidence argue against considerable sample impairment. No sign of time-dependent progression of the degradation of mitochondria was observed. For example, the V_ADP values registered as in Fig. 4 for the whole groups of antral and corpus specimens (0.453 ± 0.033 and 0.782 ± 0.056 nmol O₂·min^–1·mg^–1, n = 27, respectively) were not lower than the corresponding values of analogous parameter, V_Glut (Table 2), despite the markedly longer incubation period before ADP addition within the former protocol (35-40 min, Fig. 4) than within the protocol for V_Glut assessment (usually 5–10 min; see METHODS). On the other hand, for the groups of probes with different cytochrome c effects (<20% and 20%), the mean incubation period before addition of cytochrome c into the medium was found to be similar: 51.73 ± 1.46 (Figs. 6, A and B, bars <20%), 52.84 ± 2.43 (Fig. 6A, bar 20%), and 51.43 ± 2.4 min (Fig. 6B, bar 20%); likewise, the duration of the skinning procedure was kept constant for all mucosal probes (METHODS). In addition, as mentioned above, analysis of the 1/[ADP] vs. 1/V relationships (Fig. 5A) did not reveal the population of isolated mitochondria, characteristic of degradation of the cells. Finally, in recent studies on the function of mitochondria in human atrial cells, the positive cytochrome c effect was not observed (52) using the same protocols of cell permeabilization and oxygraphy as applied in this study. Altogether these data rule out significant nonspecific damage of the gastric mucosal specimens, at least during oxygraphy. At the same time, most of the patients had an H. pylori infection, capable of altering the processes of oxidative phosphorylation (Fig. 7) and of imposing the structural changes in mitochondria via multiple mechanisms as described above. It is therefore possible that increased permeability of MOM and impaired coupling of kinases to ANT are related to the specific effects of H. pylori and associated inflammatory reactions exerted upon mitochondrial structures. Notably, partial disintegration of cell structure, resulting from ischemia-reperfusion injury and genetic knockout of cytoskeletal proteins is also characterized by altered functions of the MOM and mitochondrial kinases (27, 28), which suggests that for these disturbances and those produced by H. pylori the impairment of the MOM represents a common stage with adverse consequences. First, it facilitates diffusion of cytoplasmic ADP into the intermembrane compartment in which excess ADP may hinder the functional coupling between mitochondrial kinases and oxidative phosphorylation (27, 47). Second, it enables mitochondrial leak of cytochrome c and kinases, these changes being causal for suppressed electron flow along the respiratory chain and for impaired intracellular energy transfer, respectively (28, 48). Thus we provide first evidence that the inflammation related to H. pylori affects the cellular energy metabolism not only by influencing the system of oxidative phosphorylation, but also by interfering with the systems of coupled reactions of kinases and ANT in the mitochondria. Because others have shown an association of gastric adenocarcinoma with suppressed expression of B-CK (21, 22), it appears that the whole system of intracellular energy transfer might be targeted by H. pylori and accompanied inflammatory factors in the pathogenesis of different gastric diseases. Recently, regulation of oxidative phosphorylation by ADP was found to be markedly affected by the changes in muscle cell contractile function and structure (4). Further research is required to elucidate whether analogous structure-function relationships exist in different cell types within the gastric mucosa.

	GRANTS

TOP ABSTRACT METHODS RESULTS DISCUSSION GRANTS REFERENCES

 
This work was supported by Estonian Science Foundation's Grant 5266, and by Grants 0182549s03 and 0182558s03 from the Estonian Ministry of Education and Research.

	ACKNOWLEDGMENTS

 
The authors thank Dr. F. N. Gellerich for valuable comments, E. Gvozdkova for technical assistance, and E. Jaigma for correcting the English.

	FOOTNOTES

 

Address for reprint requests and other correspondence: E. K. Seppet, Dept. of Pathophysiology, Faculty of Medicine, Univ. of Tartu, 19 Ravila St., 50411 Tartu, Estonia (e-mail: enn.seppet{at}ut.ee)

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.

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