Subcellular fractionation.

Livers were perfused with 37°C Krebs-Henseleit buffer (freshly added 1.3 mM CaCl₂) at a flow of 5 ml/min for 15 min, equilibrated with O₂/CO₂ (19:1) with a Silastic tubing oxygenator. Afterwards, livers were excised and washed in cold (4°C) phosphate-buffered saline. Mitochondria from whole liver were isolated according to a commercial protocol (G-Bioscience, St. Louis, MO), with slight modifications. Briefly, 500 mg of liver tissue were washed with 10 ml of ice-cold phosphate-buffered saline, before the tissue was minced with a razor blade. The minced tissue was homogenized on ice in a glass Dounce homogenizer (15 strokes, pestle A; 15 strokes, pestle B) in homogenization buffer (5 ml/g tissue). The nuclear fraction and cell debris were removed by centrifugation (1,550 g, 10 min, 4°C), and the supernatant was transferred to a new centrifuge tube. By sequential centrifugation (24,700 g, 30 min and 10 min, 4°C) of this supernatant, the mitochondria were sedimented and resuspended in suspension buffer (5 ml/g tissue), whereas the remaining supernatant (cytosolic fraction) was collected. All fractions were stored at −80°C. For the two-dimensional (2D) gel analysis, the enriched mitochondrial pellet was resuspended in a 2D gel extraction/urea lysis buffer [extraction buffer: 10 mM Tris, pH 7.6, 0.5% 3-[(3-cholamidopropyl)dimethylammonio]-1-propanesulfonate (CHAPS), freshly added PMSF, leupeptin, PIC, DTT, and phosphatase inhibitor cocktail II (Sigma); urea lysis buffer: 9 M urea, 4% CHAPS, 2% DTT, 0.1% SDS] by mixing end over end (1 ml, 30 min, 4°C). The mitochondrial suspension was centrifuged (24,700 g, 5 min, 4°C), and the crude mitochondrial enriched supernatant was transferred to a new centrifugation tube and stored at −20°C.

Hepatocyte isolation.

Hepatocytes were isolated by non-recirculating collagenase perfusion through the portal vein. Livers were perfused in situ for 5 min with Ca²⁺- and Mg²⁺-free Hank's balanced salt solution (pH 7.4) with 50 U/ml collagenase at a flow rate initiated at 8 ml/min, which was then immediately increased to 55 ml/min. The liver was excised, minced, and strained through a steel mesh and brought to a final volume of 25 ml in Williams' medium and collected by centrifugation at 50 g for 2 min at 4°C. Cells were washed three times in 25 ml of Williams' medium (50 g for 2 min at 4°C). The cell pellet was resuspended in 11 ml L15C medium (Leibovitz tissue culture medium, pH 7.4; 18 mM HEPES; 1.5 mg/ml glucose; 0.5 μg/ml insulin; 2.0 mg/ml BSA; 100 μg/ml penicillin/streptomycin) and followed by adding 10 ml Percoll solution (9 parts Percoll/1 part 10× Hanks balanced salt solution). After spinning at 50 g for 15 min at 4°C, the supernatant was removed, and the isolated hepatocytes were washed two times in 15 ml Williams' medium (50 g for 2 min at 4°C). Viability was checked by trypan blue exclusion.

2D gel electrophoresis.

Proteins from whole liver mitochondria were separated by a 2D electrophoresis, using precast immobilized pH gradient strips (IPG strips, Amersham, Piscataway, NJ) with pH ranges 4–7 (narrow range). Mitochondrial protein concentration was determined using the GenoTech Non-Interfering Protein Assay (G-Biosciences, St. Louis, MO). For isoelectric focusing, the samples were loaded on the IPG strip by in-gel sample rehydration, using a urea-thiourea mixture as solubilizing agent overnight. One-hundred fifty micrograms of protein were loaded per sample on the first-dimension gel. Isoelectric focusing on an IPG-Phor isoelectrofocusing unit (Amersham/GE healthcare, Piscataway, NJ) was conducted at 20°C, focused for 22 h [0–300 V in 1 min (gradient), 300 V for 2 h; 300–3,500 V in 2 h (gradient), 3,500 V for 20 h] for a total of 77.9 kVh. IPG strips were equilibrated three times for 15 min in freshly prepared equilibration buffer (respectively, 40 ml per equilibration; equilibration buffer: 6 M urea, 112 mM Tris-acetate, 30% vol/vol glycerol, 5% wt/vol SDS, 0.01% wt/vol bromphenol blue, adjust pH to 8.8 with acetic acid, freshly add DTT or IAA) before the second-dimension SDS-PAGE was carried out. Strips were embedded on top of 10T, 2.2C duracryl double gels (220 × 220 × 1.5 mm; Genomic Solutions, Ann Arbor, MI) after filling the chambers of the vertical SDS-PAGE unit (Investigator 2D gel running system, Genomic Solution) with appropriated buffers (anode buffer: 210 mM Tris-acetate, pH 8.9 with acetic acid; cathode buffer: 100 mM Tris, 100 mM tricine, 0.1% wt/vol SDS). The second-dimensional electrophoresis was carried out at 8°C with constant power (15 W) for 6 h. The protein spots were visualized by silver staining, using a silver stain kit (Genomic Solutions), scanned (Image Scanner II, Amersham/GE Healthcare), and digital quantified with the differential display image analysis software Z3 (Compugen, Tel-Aviv, Israel). All 2D gels were run a minimum of three independent times under each condition to ensure reproducibility.

Protein digestion and peptide mass spectrometry.

Each spot was assigned a value in parts per million corresponding to the single-spot volume as a proportion of the total spot volume of all spots in the gel, following background subtraction and removal of other artifacts. Differential expression between the groups was determined as a fold change, and proteins with the most appropriated change in expression between the groups were selected for analysis by peptide mass spectrometry (MS). Protein spots were excised, chopped, destained, and dehydrated from the gels and subjected to a tryptic digestion, as originally described by Shevchenko et al. (40) with modification as presented by Jarrold et al. (15). The extracted peptides were concentrated in a speed vac centrifuge (Speed-Vac plus, Savant, Ramsey, MN) to a final volume of 10–15 μl. Peptides were desalted and purified utilizing the C₁₈ ZipTips (Millipore, Bedford, MA). Purified peptides were eluted by pipetting up 2.5 μl of 0.3% trifluoroacetic acid in 60% vol/vol acetonitrile, followed by peptide concentration to a final volume of 0.5 μl by speed vac centrifugation. After incorporation of the concentrated peptides in 1 μl matrix solution (0.1% trifluoroacetic acid in 50% vol/vol acetonitrile + 5 mM ammonium phosphate monobasic + 5 μg/μl α-cyano-4-hydroxy-cinnamic acid), they were directly loaded onto a matrix-assisted laser desorption/ionization (MALDI) target plate (Opti-TOF 384 well plates, Applied Biosystems, Foster City, CA). MALDI-MS analysis of the respective peptides was performed on a 4800 MALDI-time-of-flight (TOF)-TOF instrument from Applied Biosystems (Foster City, CA), operated in reflector-positive mode. Proteins were subsequently identified using the MASCOT search algorithm (Matrix Science, Boston, MA) (33) from a combination of peptide mass fingerprint profiles and MS/MS sequencing data of the 10 most abundant from each digest. Criteria for protein identification included the total ion scores, a minimum of two MS/MS spectra, and the percent sequence coverage.

Western blot analysis.

Protein concentrations of subcellular fractions, either from whole liver tissue or from isolated hepatocytes, were estimated by the BCA protein assay kit (Pierce, Rockford, IL). Samples were separated in precast, denaturing 8–12% SDS-polyacrylamide gel (Pierce, Rockford, IL) and transferred to a 0.1-μm-pore nitrocellulose membrane. Nonspecific binding sites were blocked with Tris-buffered saline with 0.1% Tween 20 [TBST; 40 mM Tris (ph 7.5), 300 mM NaCl] containing either 5% nonfat dry milk or 5% BSA. Incubation of the primary antibodies [cyclooxygenase (COX) IV, cytochrome c (Cell Signaling Technology, Danvers, MA); histone H1.0, Prdx6 (Abcam, Cambridge, MA); IκB-α (Santa Cruz Biotechnology, Santa Cruz, CA)] was performed in TBST containing either 5% nonfat dry milk or 5% BSA overnight at 4°C. The membranes were washed in TBST three times for 15 min and incubated with secondary antibodies conjugated to horseradish peroxidase. Immunoreactive proteins were visualized by autoradiography, using the enhanced chemiluminescence Western Blotting Detection Reagent (Amersham, GE Healthcare Bio-Sciences).

Liver neutrophil accumulation.

Liver myeloperoxidase content was assessed by methods described elsewhere (36). Briefly, 100 mg liver tissue were homogenized in 2 ml buffer A (3.4 mmol/l KH₂HPO₄ and 16 mmol/l Na₂HPO₄, pH 7.4) for 30 s on ice. After centrifugation at 10,000 g for 20 min at 4°C, the supernatant was discarded, and the pellet was resuspended in 10 volumes of buffer B (43.2 mmol/l KH₂HPO₄, 6.5 mmol/l Na₂HPO₄, 10 mmol/l EDTA, and 0.5% hexadecyl-trimethylammonium, pH 6.0). The tissue suspension was sonicated for 30 s on ice and incubated for 2 h at 60°C. After centrifugation at 10,000 g for 5 min at 4°C, the supernatant was collected, and an aliquot was mixed with buffer C [43.3% wt/vol 3,3′,5,5′-tetramethylbenzidine, 3.2 ml N,N-dimethylformamide, 12.0 ml dH₂O, 2.6 ml buffer D (77,4 mmol/l KH₂HPO_4, 2.6 mmol/l Na₂HPO₄, 10% hexadecyltrimethyl-ammonium, add dH₂O to a final volume of 130 ml, pH 5.4), add freshly 1 μl H₂O₂] and incubated at 37°C for 15 min, and the optical density was measured at 655 nm.

Blood and tissue analysis.

Blood was obtained by cardiac puncture for analysis of serum alanine aminotransferase (ALT) as an index of hepatocellular damage. Measurements of serum ALT were made using a colorimetric diagnostic kit (Wiener Laboratorios, Rosario, Argentina), according to the manufacturer's instructions. For histological examination, liver tissues were fixed in 10% neutral buffered formalin, embedded in paraffin before cut, and stained with hematoxylin and eosin.

Fluorescence-based assay of mitochondrial respiration.

Hepatocyte mitochondria were isolated as previously outlined with minor modifications (9, 18, 43). All steps were carried out at 4°C. Briefly, 500 mg of liver were minced and washed in isolation buffer I (210 mM mannitol, 70 mM sucrose, 5 mM HEPES, 1 mM EGTA, and 0.5% fatty acid-free BSA, pH 7.4) until the homogenate was blood free. Five volumes of isolation buffer I were added, and the tissue homogenized using a smooth glass grinder with Teflon pestle driven by a power drill. The homogenate was then adjusted to eight volumes of isolation buffer I and centrifuged at 700 g for 10 min at 4°C. The supernatant was filtered through two layers of cheesecloth and recentrifuged for 10 min at 14,000 g to precipitate the mitochondrial fraction. The supernatant was discarded; mitochondria were washed by resuspension in 4 ml of isolation buffer I and centrifuged at 10,000 g for 10 min at 4°C. This washing step was repeated in isolation buffer II (210 mM mannitol, 70 mM sucrose, 10 mM MgCl₂, 5 mM K₂HPO₄, 10 mM 3-(N-morpholino)propanesulfonic acid, and 1 mM EGTA, pH 7.4). Finally, mitochondria were resuspended in 450 μl isolation buffer II. Protein measurements were preformed to adjust equal amounts of mitochondrial proteins. One-nanomole A65N-1 oxygen probe (Luxcel Bioscience, Cork, Ireland), supplied as dry reagent, was reconstituted in 1 ml of respiration buffer (250 mM sucrose, 15 mM KCl, 1 mM EGTA, 5 mM MgCl₂, and 30 mM K₂HPO₄, pH 7.4) and diluted to a concentration of 100 nM. One-hundred microliters of this solution were transferred into a 96-well plate (100 pmol of probe per well). Fifty microliters of the mitochondrial proteins were added to each well, followed by 50 μl of substrate (12.5:12.5 mM glutamate-malate final concentration) without or with ADP (1.65 mM final concentration). As positive control, respiratory chain uncoupling was tested by using carbonyl cyanide 4-(trifluoromethoxy) phenyldydrazone (final concentration 100 nmol/mg protein), dissolved in dimethyl sulfoxide (final dimethyl sulfoxide content was not more than 0.5% vol/vol). Finally, 100 μl of heavy mineral oil were added to each well to seal the samples from ambient oxygen. Measurement was done in a Victor³V (PerkinElmer precisely, 1420 Multilabel counter) at 30°C for 90 min in a time-resolved fluorescence mode. Instrument settings were as follows, 340/642 nm excitation/emission filters, a delay of 30 μs, and a measurement window of 100 μs. After completion of fluorescence measurements, time profiles of fluorescence intensity were analyzed using WorkOut2 (PerkinElmer) software. Rates of oxygen consumption based on the known relationship between probe fluorescence quenching and oxygen concentration were determined (17). Briefly, fluorescence traces were converted into oxygen concentration profiles using the following transformation:

where [O₂]_a is oxygen concentration in air-saturated buffer (235 μM at 30°C); I(t), I_o, and I_a are fluorescence signal of the probe at time t, signal in air-saturated buffer (baseline signal without enzyme), and signal in deoxygenated buffer (maximal signal), respectively. Rates of change of dissolved oxygen were subsequently determined from the initial slopes of these concentration profiles, similar to the electrode system.

Mitochondrial respiration and energy coupling.

Mitochondrial oxygen consumption was measured polarographically with a computer-controlled Clark-type oxygen electrode (Hansatech Instruments, Norfolk, UK). The respiratory mixture, consisting of 0.5 ml of a KCl respiratory buffer [140 mM KCl, 0.1 mM EDTA, 2.5 mM KH₂PO₄, 2.5 mM MgCl₂, and 0.05% bovine serum albumin, in 5 mM HEPES, pH 7.4 (KOH)] and 150 μg of mitochondrial protein were equilibrated at 37°C under constant stirring. Substrate-stimulated state 4 respiration (ADP limited) was determined after adding 3 mM glutamate/3 mM malate or 6 mM sodium succinate. The rate of state 3 respiration was then determined following the addition of 0.2 mM ADP. The respiratory control ratio (RCR) was calculated as the ratio of state 3 to state 4 respiration.

Measurement of mitochondrial reactive oxygen using luminol.

H₂O₂-induced luminol chemiluminescence was measured as described elsewhere (37), using a Berthold Autolumat Plus luminometer. Luminol will react with H₂O₂ and peroxynitirite, but not with superoxide (38). H₂O₂ specificity is determined by inhibiting chemiluminescence with catalase. The reaction mixture is composed of 100 μg of mitochondrial protein, 5 μM luminol, and 10 μg/ml horseradish peroxidase in a final volume of 1.0 ml KCl respiratory buffer. Chemiluminescence was initiated by the addition of either 3 mM glutamate/3 mM malate or 6 mM sodium succinate, and monitored at 37°C. The H₂O₂ luminescence signal was completely quenched by 500 units catalase/ml; values shown are catalase-inhibited chemiluminescence values.

Subcellular expression of Prdx6 in whole liver tissue and hepatocytes.

To determine the subcellular localization of Prdx6 and to determine whether this expression pattern is altered by I/R, we analyzed whole liver cytoplasmic and mitochondrial expression of Prdx6 by Western blot. As shown in Fig. 2A, Prdx6 expression was found uniformly in the cytoplasm. Interestingly, we found that, after ischemia or I/R, Prdx6 could be detected in the mitochondrial fraction, indicating trafficking of Prdx6 from the cytoplasm to the mitochondria. To ensure the physical integrity of the hepatic mitochondria isolated from postischemic livers, Western blot for cytochrome c was performed. These studies demonstrated that isolated mitochondria were intact, as no leakage of cytochrome c to the cytoplasm was detected (Fig. 2B).

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Fig. 2.

Hepatic peroxiredoxin (Prdx) 6 expression in cytoplasmic and mitochondrial compartments during I/R. A: cytoplasmic (c) and mitochondrial (m) protein fractions were isolated from livers of mice undergoing sham surgery, 90 min of ischemia (90/0), and 90/1, and immunoblotted for Prdx6. Data are representative of three independent experiments. B: the integrity of isolated mitochondria was determined by immunobloting cytoplasmic and mitochondrial fractions for cytochrome c. Data are representative of three independent experiments.

Because derangement of mitochondrial function in hepatocytes is the trigger for cell death, we next examined Prdx6 expression in subcellular fractions of hepatocytes isolated during I/R. In hepatocytes from sham-operated control mice, Prdx6 was found primarily in the cytoplasmic compartment with minimal Prdx6 detected in mitochondria (Fig. 3). However, after ischemia or I/R, Prdx6 expression in the cytoplasm was lost, and Prdx6 expression in mitochondria was markedly increased (Fig. 3). COX IV staining indicated equal loading of mitochondrial protein. The purity of the isolated fractions was done in the same way as described for whole liver tissue, and no contamination of the mitochondrial or cytoplasmic fractions was detectable (data not shown). Collectively, these data suggest that ischemic stress to hepatocytes induces shuttling of Prdx6 from the cytoplasm to the mitochondria.

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Fig. 3.

Hepatocyte Prdx6 expression in cytoplasmic and mitochondrial compartments during I/R. Cytoplasmic and mitochondrial protein fractions were isolated from livers of mice undergoing sham surgery, 90/0, 90/1, and 90 min of ischemia and 4 h of reperfusion (90/4), and immunoblotted for Prdx6. The same subcellular fractions were immunoblotted for COX IV to serve as a loading control, as well as an index of mitochondrial integrity. Data are representative of three independent experiments.

Prdx6 protects against liver injury induced by I/R.

Our data demonstrate that, in hepatocytes, Prdx6 traffics from the cytoplasm to mitochondria during I/R. It is well established that mitochondrial function dictates hepatocyte survival. To determine whether the mitochondrial trafficking of Prdx6 in hepatocytes during I/R has an effect on hepatic injury, we examined the injury response of wild-type (WT) and Prdx6-knockout (KO) mice to I/R in vivo. Mice were subjected to 90 min of ischemia followed by 8 h of reperfusion, which is known to cause severe hepatocellular injury. Prdx6-KO mice had significantly greater liver injury, as determined by serum levels of ALT (Fig. 4A). Despite this increase in liver injury, Prdx6-KO mice had significantly less neutrophil accumulation, as measured by liver content of myeloperoxidase (Fig. 4B). These biochemical data were confirmed by histopathological analysis. Sham-operated WT and Prdx6-KO mice displayed normal liver architecture (Fig. 4C). After I/R in WT mice, there was marked neutrophilic inflammation and hepatocyte necrosis (Fig. 4C). However, in the Prdx6-KO mice, there was less evidence of neutrophilic infiltrates, yet hepatocellular necrosis was more severe than in WT mice (Fig. 4C). To determine if the increased liver injury observed might be a result of increased apoptosis, we stained liver sections for active caspase-3. There was no difference in the amount of staining for active caspase-3 in livers from WT and Pdx6-KO mice (data not shown). These data demonstrate that Prdx6 is an important regulator of the hepatic injury response to I/R.

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Fig. 4.

Prdx6 protects against hepatic I/R injury. Wild-type (WT) and Prdx6-knockout (Prdx6-KO) mice were subjected to 90 min of ischemia followed by 8 h of reperfusion. A: hepatocellular injury was determined by measuring serum levels of alanine aminotransferase (ALT). B: neutrophil accumulation was determined by liver content of myeloperoxidase (MPO). Values are means ± SE with n = 3 per group. *P < 0.05 compared with sham. C: Liver histology. Normal hepatic architecture was observed in sham-operated WT mice and Prdx6-KO mice. After I/R, livers from WT mice had large areas of necrosis with neutrophilic infiltration, whereas livers from Prdx6-KO mice showed more widespread necrosis with little evidence of neutrophil accumulation. Original magnification was ×100.

Mitochondrial Prdx6 stabilizes mitochondrial respiratory chain function during liver I/R.

To determine if the increased liver injury observed in Prdx6-KO mice was attributable to increased mitochondrial dysfunction as a result of the loss of mitochondrial Prdx6, respiratory activities of liver mitochondria from WT and Prdx6-KO mice were evaluated in the presence of glutamate/malate (substrates for complex I) or succinate (substrate for complex II) and ADP. The RCR is a ratio of maximal respiration (state 3) to basal respiration (state 4) and represents an index of mitochondrial coupling and, therefore, function. After stimulation with glutamate/malate, mitochondria from Prdx6-KO mice showed a higher RCR baseline (Fig. 5A). Despite this, mitochondria from Prdx6-KO mice showed a precipitous decrease in RCR over the time course of I/R. In contrast, mitochondria from WT mice showed an initial decrease in RCR after ischemia or ischemia and 1 h of reperfusion, but then recovered by 4 h of reperfusion (Fig. 5A). A similar phenomenon was observed in mitochondria stimulated with succinate (Fig. 5B).

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Fig. 5.

Effect of I/R on respiratory control ratio (RCR) in liver mitochondria from WT and Prdx6-KO mice. A: stimulation of complex I with glutamate/malate. B: stimulation of complex II with succinate. Values are means ± SE with n = 3 per group. *P < 0.05.

To further explore the importance of mitochondrial Prdx6 in stabilizing mitochondrial function, we examined mitochondrial oxygen consumption using a kinetic assay employing a long-decay, phosphorescent, oxygen probe (9). Because we found that complex I was more affected by the loss of Prdx6, we only used glutamate/malate as a substrate in this assay. As shown in Fig. 6, mitochondria from WT and Prdx6-KO mice had similar basal (state 4) oxygen consumption after sham surgery or I/R (Fig. 6). ADP-stimulated (state 3) oxygen consumption was similar between mitochondria from sham-operated WT and Prdx6-KO mice (Fig. 6). After ischemia, oxygen consumption by mitochondria from Prdx6-KO mice greatly exceeded that from WT mice. After ischemia and 1 h of reperfusion, oxygen consumption was again similar between WT and Prdx6-KO mitochondria (Fig. 6).

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Fig. 6.

Effect of I/R on oxygen consumption in liver mitochondria from WT and Prdx6-KO mice. Kinetic analysis of oxygen consumption was conducted by fluorescence analysis of glutamate/malate-driven respiration of liver mitochondria from mice undergoing sham surgery, 90/0, and 90/1. Values are means ± SE with n = 3 per group. *P < 0.05 compared with Prdx6-KO.