©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
Activity of the Mitochondrial Multiple Conductance Channel Is Independent of the Adenine Nucleotide Translocator (*)

(Received for publication, September 1, 1995; and in revised form, November 8, 1995)

Timothy A. Lohret (1) (3) Robert C. Murphy (1) (4) Tomas Drgoñ (5) Kathleen W. Kinnally (1) (2)(§)

From the  (1)Division of Molecular Medicine, Wadsworth Center, New York State Department of Health, Albany, New York, 12201-0509, Departments of (2)Biomedical Sciences and (3)Biological Sciences, University at Albany, State University of New York, Albany, New York, 12222, (4)Biology Department, Rensselaer Polytechnic Institute, Troy, New York, 12180 and (5)Department of Biochemistry, Commenius University, Bratislava, Slovak Republic 84215

ABSTRACT
INTRODUCTION
MATERIALS AND METHODS
RESULTS
DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES

ABSTRACT

The functional relationship between the adenine nucleotide translocator (ANT) and the mitochondrial multiple conductance channel (MCC) was investigated using patch-clamp techniques. MCC activity with the same conductance, ion selectivity, voltage dependence, and peptide sensitivity could be reconstituted from inner membrane fractions derived from mitochondria of ANT-deficient and wild-type Saccharomyces cerevisiae. In addition, the MCC activity of mouse kidney mitoplasts was unaffected by carboxyatractyloside, a known inhibitor of ANT and inducer of a permeability transition. These results suggest that MCC activity is independent of ANT.


INTRODUCTION

Patch-clamp experiments on mitoplasts (mitochondria with the inner membrane exposed) have detected a multiple conductance channel, MCC (^1)(also referred to as mitochondrial megachannel, MMC), which is activated by calcium(1, 2, 3, 4, 5, 6) . This multisubstate channel activity is voltage-dependent and has a peak conductance of 1-1.5 nanosiemens (see (2) and (4) for recent reviews). Szabó and Zoratti (5) have proposed that MCC may be responsible for a permeability transition in mitochondria. Halestrap and Davidson (7) have postulated that the adenine nucleotide translocator (ANT) is intrinsic to a permeability transition. Recently, Zoratti and Szabó(4) have speculated on the possibility that MCC may be associated with a dimer of ANT plus other proteins.

The protein(s) responsible for MCC activity have not been identified. However, it is possible that MCC may be associated with a membrane transporter like ANT since many transporters display channel activity when reconstituted in bilayers and proteoliposomes. These transporters include the (Na/K)-ATPase, the chloroplast triose phosphate/phosphate translocator, and members of the ATP binding cassette superfamily of transporters, e.g. cystic fibrosis transmembrane conductance regulator and multidrug-resistant transporters(8, 9, 10, 11, 12, 13, 14) . In fact, channel activity similar to that of MCC has been reported in black lipid membranes fused with proteoliposomes containing protein fractions of ANT(15) . Possible relationships between MCC and transporters can now be examined by using deletion mutants of mitochondrial transporters in yeast. Unfortunately, the other dominant inner mitochondrial membrane channel (mitochondrial centum picosiemen channel) has not yet been detected in yeast(16) .

In the present work, we have used patch-clamp techniques to compare the MCC activity in proteoliposomes reconstituted with mitochondrial inner membranes from ANT-deficient and wild-type strains of Saccharomyces cerevisiae. In addition, we have applied similar techniques to mouse kidney mitoplasts to see whether MCC activity is affected by carboxyatractyloside, which is a specific inhibitor of ANT(17) .


MATERIALS AND METHODS

Mitochondria, Mitoplast, and Proteoliposome Preparations

Mouse kidney mitochondria were isolated as described previously(18) , and mitoplasts were prepared using the French press method (at 2000 p.s.i.) of Decker and Greenawalt(19) . Mitochondria from S. cerevisiae strain M3 (wild type, graciously provided by M. Forte, Vollum Institute) and strain JL-1-3 (a triple mutant in which all three genes (AAC1, AAC2, AAC3) encoding mitochondrial ANT have been disrupted) (20) were isolated by a modification of the method of Daum et al.(21) . In general, yeast channel activities were studied after reconstitution into proteoliposomes. Isolated yeast mitoplasts (prepared by French press) were osmotically lysed and spun on a sucrose gradient according to the method of Mannella(22) . Pellets from the gradient spin were used as inner membranes, which were reconstituted into giant proteoliposomes using the dehydration-rehydration method of Criado and Keller (23) in 0.15 M KCl, 5 mM HEPES, pH 7.4, as described previously(6, 16) . Inner membrane yields were 10 and 2.5 mg of protein from overnight cultures of 20 g (2 liters) and 17 g (1.5 liters) of strains M3 and JL-1-3 cell pellets, respectively. Approximately 10% of each inner membrane preparation (0.25-1 mg of protein) was added to liposomes (5 mg of Sigma type IV-S soybean L-alpha-phosphatidylcholine) for a typical reconstitution.

Patch Clamping

The procedures and conditions used for patch clamping mitoplasts and proteoliposomes are essentially the same as previously reported(18, 24) . The reported voltage is that of the mitochondrial matrix in inside-out excised patches from mitoplasts, where V = V - V. Voltages are reported relative to the bath for proteoliposome patches since the orientation of MCC (as indicated by voltage dependence and kinetics) is the same as in mitoplasts. Open probability is calculated as the fraction of the total time spent in the fully open state from amplitude histograms using the PAT program (Strathclyde Electrophysiological Software, courtesy of J. Dempster, University of Strathclyde, UK). All yeast experiments were in done in 0.15 M KCl, 5 mM HEPES, 1 mM EGTA, 1.05 mM CaCl(2) (10M free Ca), pH 7.4. Selectivity was estimated from the reversal potential with a 5:1 KCl gradient as described previously (16) . The level of MCC activity in mammalian mitoplasts was varied by exposure to calcium as in (3) and the patching media as indicated in Table 1.



Effectors

Peptides were prepared by the Wadsworth Center's peptide synthesis core facility on an Applied Biosystems 431A automated peptide synthesizer as described previously(6) . The targeting peptides used were the amino termini of cytochrome oxidase subunit VI (^1MLSRAIFRNPVINRTLLRAR) and subunit IV (^1MLSLRQSIRFFKY) of S. cerevisiae and subunit IV (^3RAPALRRSIATTVVRCNAET) of Neurospora crassa. The control peptide was the amino terminus from N. crassa voltage-dependent anion-selective channel (^1MAVPAFSDIAKSANDLLNKD). Carboxyatractyloside (Sigma) was included in the medium in the patch pipette (and usually the bath) at concentrations of 5 or 10 µM. The presence or absence of carboxyatractyloside was alternated every 3-5 patches within each preparation of mammalian mitoplasts.

Verification of Phenotypes by Western Blot Analysis

Western blot analysis was performed on both wild-type and ANT-deficient purified mitochondrial inner membranes. Samples (10 µg of protein) were boiled in SDS-polyacrylamide gel electrophoresis sample buffer, electrophoresed in 14% polyacrylamide gel, and blotted onto a polyvinylidene difluoride membrane (Novex, San Diego, CA). Samples were then probed with anti-ANT antibodies recognizing all three isoforms of ANT (graciously provided by J. Kolarov and I. Hapala) and visualized with a horseradish peroxidase-coupled second antibody (Pierce) with diaminobenzidine as a substrate(25) .


RESULTS

MCC Is Present in ANT-deficient Yeast

Patch-clamp techniques were used to characterize the MCC activity in proteoliposomes containing mitochondrial inner membranes from a wild-type strain of yeast and a strain in which the three ANT genes were disrupted. Western blot analysis confirmed the absence of ANT in the inner membranes prepared from the later strain as shown in Fig. 1. Fig. 2illustrates typical channel activity detected in proteoliposomes derived from the ANT-deficient strain (n = 8 patches). The peak conductance state (1.1 nanosiemens in Fig. 2) and half-open substate are typical of MCC transitions observed in preparations from wild-type yeast(6, 16) . MCC activity from the ANT-deficient strain is voltage-dependent, occupying near-peak conductance levels in the potential range between -40 mV and +20 mV. At larger amplitude transmembrane potentials of either polarity, the channel tends to occupy lower conductance levels including a low noise closed state (occurring at +40 mV in Fig. 2). This voltage-dependent behavior is the same as that of reconstituted MCC from wild-type strains of yeast(2, 6, 16) .


Figure 1: ANT is absent in AAC1, AAC2, AAC3 deletion mutant. Western blot analysis using an antibody recognizing all three isoforms of ANT was performed on mitochondrial inner membranes. The blot shows the presence of ANT in membranes from wild-type yeast (lane 1) and the absence of ANT in membranes from ANT-deficient (lane 2) yeast mitochondria.




Figure 2: MCC activity is present in ANT-deficient yeast. A, current traces of MCC were recorded at various voltages from an excised patch from a proteoliposome reconstituted with mitochondrial inner membranes isolated from ANT-deficient yeast. Data were bandwidth-limited to 2 kHz and sampled at 5 kHz. Total amplitude histograms of current traces at -40 mV (B) and 30 mV (C) (bin width, 0.4 pA; duration, 15-20 s) show the occupancy of open (O), substate (S), and closed (C) conductance levels.



No significant differences between the MCC activity of wild-type and ANT-deficient yeast were resolved. MCC activity of the ANT-deficient strain is slightly cation-selective (P/P approx 6, n = 2, data not shown) like that of the wild-type strain (P/P approx 6, (16) ). Peptides whose sequences target precursor proteins to the mitochondrial inner membrane specifically induce a transient blockade of MCC from the ANT-deficient strain (n = 7 patches) as previously reported for MCC from the wild-type strain (6) (Fig. 3). Furthermore, the frequency of recording MCC is about the same from proteoliposomes from the wild-type (75%, n = 12 patches) and ANT-deficient (88%, n = 8 patches) yeast strains. We also noted that the 50 picosiemens channel activity often detected in wild-type yeast proteoliposomes (16) was also present in the ANT-deficient yeast proteoliposomes (data not shown).


Figure 3: MCC activity from ANT-deficient yeast is peptide sensitive. A, current traces show the transient blockade of MCC in the presence of 50 µM targeting peptide (amino terminus of yeast cytochrome oxidase subunit VI). B, amplitude histograms show a shift in the occupation of conductance levels in the presence (box) and absence () of the peptide. Other conditions are the same as in Fig. 2.



Mammalian MCC Is Not Affected by Carboxyatractyloside, an ANT Inhibitor

Carboxyatractyloside stabilizes the nucleotide binding site of ANT on the cytoplasmic side of the inner membrane, thereby blocking the exchange of matrix ATP and cytoplasmic ADP (K(i) approx 10M)(17) . The effect of this ANT inhibitor on MCC activity was determined in mouse kidney mitoplasts. As shown in Table 1, the frequency of recording MCC was not changed by the presence of carboxyatractyloside under a variety of conditions. That is, carboxyatractyloside does not appear to activate MCC under low calcium conditions that normally favor quiescent MCC(3) . Likewise, this ANT inhibitor does not appear to inhibit MCC activated by calcium. As shown in Table 1, the seal resistance was unchanged by the presence of carboxyatractyloside, indicating that there was no masking of MCC in a stabilized open state. (If MCC were immobilized in an open state, resistance would be below 0.5-1 gigaohm). The studies were restricted to the potential range of ±30 mV to avoid voltage activation of MCC(26) . (In general, the presence of MCC in patches scored inactive was verified by activation of MCC by higher voltages (±60-100 mV) in the presence and absence of carboxyatractyloside.)


DISCUSSION

ANT Is Not Responsible for MCC Activity

The protein(s) responsible for MCC have not yet been identified but Zoratti and Szabó(4) have speculated that this channel activity might be associated with a dimer of the transport protein ANT (plus other proteins). Tikhonova et al.(15) detected channel activity similar to that of MCC in black lipid membranes fused with proteoliposomes containing purified fractions of ANT after mersalyl addition. In addition, mersalyl induced a high conductance pathway in the proteoliposomes that was not sensitive to carboxyatractyloside. Tikhonova et al.(15) suggest that mersalyl may modify ANT so that it can operate as a channel and suggest that ANT may function as a permeability transition pore-forming protein. Similarly, Dierks et al.(27) report mersalyl induces an ATP efflux from proteoliposomes co-reconstituted with ANT and the aspartate/glutamate carrier. This efflux was inhibited 50% by concentrations of carboxyatractyloside that also eliminated ANT-mediated nucleotide exchange (27) but had no effect on aspartate efflux.

We used a molecular genetics approach to test the hypothesis that ANT was responsible for MCC activity. This has advantages over biochemical approaches, which may be compromised or confounded by trace contamination by channel proteins that are detectable with patch-clamp techniques. Channel activity with the same conductance, ion selectivity, voltage dependence, and peptide sensitivity as MCC was reconstituted from inner membrane fractions derived from mitochondria of ANT-deficient and wild-type yeast strains. These results strongly indicate that ANT is not responsible for MCC. This conclusion was supported by experiments which showed carboxyatractyloside, a known inhibitor of ANT and an activator of a permeability transition, had no effect on mammalian MCC. However, this work does not eliminate the possibility that ANT may have channel activity unrelated to MCC.

MCC and the Mitochondrial Permeability Transition

A permeability transition can be induced in mitochondria by calcium and a trigger, e.g. phosphate. Similarly, carboxyatractyloside is known to induce a permeability transition in mitochondria(7, 28) . Furthermore, a model has been proposed in which the c conformation of ANT (favored by carboxyatractyloside) is integral to a permeability transition(7) . Szabó and Zoratti have proposed that MCC activity is responsible for a permeability transition (5) since they share many characteristics including estimated pore size and pharmacology (see (2) and (4) for recent reviews). However, it is not likely MCC is associated with the permeability transition induced by carboxyatractyloside since, in this study, MCC activity was insensitive to this transition inducer. This apparent conflict may, however, be resolved since studies indicate that the induction of the permeability transition by carboxyatractyloside may be indirect by modifying adenine nucleotide levels(4, 29) .

The diversity of permeability transition effectors leads one to speculate that more than one high permeability pathway may be involved in these transitions. For example, cyclosporine inhibits the calcium-induced transition but not the butylated hydroxytoluene-induced transition(30) . If multiple pathways exist, our findings suggest MCC is not responsible for the permeability pathway induced by carboxyatractyloside.

Conclusions

Reconstituted MCC activity is the same in yeast lacking all three ANT genes as it is in the wild type. In addition, mammalian MCC is not affected by carboxyatractyloside, a known inhibitor of ANT. These findings indicate that the inner membrane translocator ANT is not responsible for the multiple conductance channel activity.


FOOTNOTES

*
This study was supported by National Science Foundation Grant MCB9117658. The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

§
To whom reprint requests should be made: Wadsworth Center, New York State Dept. of Health, Empire State Plaza, P. O. Box 509, Albany, NY 12201-0509.

(^1)
The abbreviations used are: MCC, multiple conductance channel; ANT, adenine nucleotide translocator.


ACKNOWLEDGEMENTS

We thank Dr. James Dias and the Wadsworth Center's peptide synthesis core facility for synthesis of peptides. We thank Dr. Michael Forte for the yeast strain M-3 and Drs. Jordan Kolarov and Ivan Hapala for the ANT antibodies. We thank Dr. Enrico Cabib for his support of T. D. at NIDDK-LBM, NIH. We thank Drs. Patricia Sokolove, Richard Zitomer, Henry Tedeschi, and especially Carmen Mannella for support, discussions, and review of this manuscript.


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©1996 by The American Society for Biochemistry and Molecular Biology, Inc.