(Received for publication, March 28, 1997, and in revised form, May 13, 1997)
From the Institut für Physiologische Chemie, Universität München, Goethestraße 33, 80336 München, Federal Republic of Germany
The requirement of mitochondrial hsp70 (mt-hsp70) for the import of a series of preproteins containing hydrophobic sorting signals into isolated yeast mitochondria was investigated. Here we demonstrate that the presence of such a sorting signal in proximity to the N-terminal matrix-targeting sequence of a preprotein can secure a translocating polypeptide chain in the import channel in a manner that does not require mt-hsp70 activity. Trapping the translocating chain in this fashion leads to efficient processing by the mitochondrial processing peptidase and to complete translocation across the outer mitochondrial membrane into the intermembrane space. These mt-hsp70-independent effects appear to be exerted at the level of the inner membrane through an interaction of the hydrophobic core of the sorting signal with component(s) of the translocase of the inner membrane. Hydrophobic sorting signals of inner membrane proteins inserted into the membrane from the matrix, as well as those of intermembrane space proteins, are capable of causing this mt-hsp70-independent stabilization, demonstrating that this phenomenon is not unique to those preproteins normally sorted to the intermembrane space.
The import of nuclear encoded preproteins into the mitochondrial
matrix involves the coordinated action of translocation machineries in
both the outer and inner mitochondrial membranes (1-3). The majority
of these preproteins are targeted to the mitochondria by N-terminal
targeting sequences that are processed in the matrix by the
mitochondrial processing peptidase (MPP)1
(4, 5). In addition to their targeting function, presequences initiate
translocation across the inner membrane via the TIM
(translocase of the inner membrane)
machinery in a -dependent manner (6-12). Binding of
the molecular chaperone mt-hsp70, together with TIM44, a component of
the TIM machinery, serves to hold the presequence upon its exposure to
the matrix and thus confers unidirectionality on the import process
(13, 14). Studies with matrix-targeted preproteins suggested that
binding of mt-hsp70 to the preprotein is the only or major force for
achieving vectorial movement at the initial steps of import. Supporting
this, retrograde movement of the translocating polypeptide was observed
if bound mt-hsp70 was released (12, 15, 16). On the other hand, the
activity of mt-hsp70 was observed not to be required to initiate
translocation of some preproteins targeted to the inner membrane
(17-20).
To study the mechanism by which mt-hsp70 function is bypassed, we analyzed the import of preproteins either destined for the inner membrane (which are first imported into the matrix; see below) or targeted to the intermembrane space. These preproteins all contain hydrophobic sorting signals. Their import in the presence or absence of functional mt-hsp70 was investigated. The precursor proteins chosen consisted of N-terminal segments of either pre-subunit 9 of the F1F0-ATPase or precytochrome b2 fused to mouse dihydrofolate reductase (DHFR). The pre-subunit 9 chimera included the first transmembrane domain of subunit 9 fused to DHFR (pSu9-(1-112)-DHFR) and attains an Nout-Cin topology across the inner membrane in an export event following initial import into the matrix (20). Cytochrome b2, on the other hand, is targeted to the intermembrane space by a cleavable N-terminal bipartite presequence that is initially processed by MPP. According to recent evidence, the sorting signal targets cytochrome b2 along a sorting pathway that involves at least partial passage through the matrix (21). This import pathway differs, however, from that of matrix-targeted preproteins, as it appears to disengage from mt-hsp70 machinery at an early stage of the import process (22).
In this paper, we report that the hydrophobic sorting signal of a preprotein, when in proximity to a matrix-targeting sequence, can guarantee the maintenance of a translocating polypeptide in the TIM channel in the apparent absence of mt-hsp70 activity, thereby efficient MPP processing, as well as translocation across the outer membrane, takes place under conditions when further translocation across the inner membrane is blocked. Sorting signals of both a matrix-targeted protein and an intermembrane space protein were capable of mediating this mt-hsp70-independent securing of translocating polypeptides in the TIM machinery. The common denominator for maintaining a preprotein in the TIM channel is therefore a suitably positioned hydrophobic core rather than a sorting signal specific for one mitochondrial subcompartment over another. We propose that hydrophobic segments retard the sliding of a translocating chain in the import channel to facilitate recognition and lateral exit of those preproteins that become inserted into the inner membrane.
Saccharomyces cerevisiae wild-type strain D273-10B was grown in lactate medium (23) at 30 °C, whereas the temperature-sensitive mutant of mt-hsp70, ssc1-3 (PK83), and its corresponding wild type (PK82) (24) were grown at 24 °C. Mitochondria were isolated as described previously (23, 27).
Precursor ProteinsDNA encoding precursor proteins was transcribed with SP6 RNA polymerase as described previously for the cytochrome b2-derived precursors (18, 25) and the pSu9-DHFR fusion proteins (15). All precursor proteins were then synthesized in rabbit reticulocyte lysate (Promega) in the presence of [35S]methionine (26).
Import into Mitoplasts and MitochondriaIsolated mitochondria were converted to mitoplasts prior to import as follows. Mitochondria were diluted 10-fold in 10 mM potassium Pi buffer and incubated for 20 min at 0 °C prior to reisolation and resuspension in SEM buffer (250 mM sucrose, 2 mM EDTA, 10 mM MOPS, pH 7.2).
Import was performed at 25 °C in the following buffer: 220 mM sucrose, 80 mM KCl, 10 mM MOPS/KOH, pH 7.2, 3% bovine serum albumin (w/v) 25 mM potassium phosphate, 5 mM MgOAc, and 1 mM MnCl2. Import mixtures contained 2 mM NADH, 3 µM hemin, 0.3 mg/ml mitochondrial protein, and 1% (v/v) reticulocyte lysate containing the radiolabeled precursor proteins. Samples were treated with proteinase K (50 µg/ml) for 30 min at 0 °C under either non-swelling or hypotonic swelling conditions (see below) (27). Samples were analyzed by SDS-PAGE and immunoblotting onto nitrocellulose. The efficiency of swelling of the mitochondria was assessed following immunodecoration of the blot with antisera against endogenous cytochrome c peroxidase (soluble intermembrane space protein) and Mge1p (matrix-localized protein). Swelling in each case was >95% efficient, whereas the integrity of the inner membrane was not perturbed (data not shown).
Methotrexate Arrest of DHFR Fusion ProteinsTo stall the import of the various DHFR fusion proteins with methotrexate/NADPH, translation of the radiolabeled proteins was performed at 25 °C in the presence of 1 µM methotrexate. The reticulocyte lysates were diluted in import buffer containing 1 µM methotrexate and 1 mM NADPH and incubated for 5 min at 0 °C followed by 5 min at 25 °C prior to the addition of mitochondria.
Depletion of Matrix ATPIsolated mitochondria were depleted of their free matrix ATP by treatment with oligomycin and carboxyatractyloside as described previously (28). When matrix ATP levels were to be restored in depleted mitochondria following an import reaction, mitochondria were incubated in import buffer with oligomycin (20 µM) and apyrase (40 units/ml) for 3 min at 25 °C, and the carboxyatractyloside was omitted. (This depletion procedure resulted in a >90% import inhibition of the matrix-targeted preprotein pSu9-(1-69)-DHFR (data not shown).) Matrix ATP was replenished by incubating the reisolated and washed mitochondria in the presence of 5 mM succinate, 5 mM malate, 2 mM ATP, and 2 mM NADH.
Chemical Cross-linking and Co-immunoprecipitation AnalysispSu9-(1-112)-DHFR was arrested as a methotrexate translocation intermediate across the inner membrane in mitoplasts. Chemical cross-linking with disuccinimidyl suberate (200 µM) and immunoprecipitation of the resulting cross-linked adducts were performed as described previously (11).
MiscellaneousProtein determination and SDS-PAGE were performed according to the published methods of Bradford (29) and Laemmli (30), respectively. The detection of proteins after blotting onto nitrocellulose was performed using the ECL detection system (Amersham Corp.).
To study the ability of hydrophobic
sequences in preproteins to interact with the TIM translocation
channel, the import of a number of precursor proteins was analyzed: the
cytochrome b2-derived preproteins
pb2-(1-76)-DHFR,
pb2-(1-85)-DHFR, and
pb2-(1-109)-DHFR and the matrix-targeted inner
membrane protein pSu9-(1-112)-DHFR (Fig.
1A). Import was performed initially in the
presence of methotrexate to arrest the DHFR domain in a tightly folded
state at the surface of the outer membrane and thereby allow only
translocation of the N-terminal region of the precursor across the
inner membrane. The positions of the hydrophobic segments in the
various preproteins relative to MPP processing sites are depicted in
Fig. 1A.
Accumulation of intermediates processed by MPP was used as an indicator for the transfer of the matrix-targeting sequence across the inner membrane into the matrix. When imported into wild-type mitochondria, all precursors arrested with methotrexate were efficiently processed by MPP and were reisolated with the mitochondria (Fig. 1B). Upon import into mitochondria containing inactivated mt-hsp70 from the temperature-sensitive ssc1-3 mutant (24), the processing of pb2-(1-76)-DHFR, pb2-(1-85)-DHFR, and pSu9-(1-112)-DHFR by MPP was inhibited. In contrast, pb2-(1-109)-DHFR was efficiently processed to its intermediate-size form in the absence of mt-hsp70 activity (Fig. 1B). Thus, despite that all three precursors contain hydrophobic segments, only methotrexate-arrested pb2-(1-109)-DHFR can be accumulated as an MPP-processed translocation intermediate in intact mitochondria in the absence of functional mt-hsp70. On the other hand, all of these methotrexate-arrested preproteins can be accumulated as MPP-processed translocation intermediates upon import into mitoplasts in the absence of functional mt-hsp70 (data not shown). These findings suggest that the hydrophobic segment must extend at least to the inner membrane to secure stabilization of a translocation intermediate in an mt-hsp70-independent manner.
Matrix ATP Requirement for the Import and Sorting of PreproteinsDepletion of matrix ATP levels impairs the
ATP-dependent activity of mt-hsp70 and leads to an almost
complete block of import of hydrophilic matrix-targeted proteins (13,
19, 28). The cytochrome b2-derived precursor
proteins analyzed were efficiently processed by MPP and were imported
to a protease-resistant location in the mitochondria in a matrix
ATP-independent manner (Fig. 2, upper panel,
+ATP versus ATP). A similar ATP independence of import was
obtained for the pSu9-(1-112)-DHFR protein, despite that it is a
matrix-targeted protein (Fig. 2, lower panel, +ATP versus
ATP). This is in marked contrast to the hydrophilic
matrix-targeted precursor protein pSu9-(1-69)-DHFR, where import was
strictly matrix ATP-dependent (Fig. 2, lower
panel). Subfractionation of the mitochondria by hypotonic swelling
revealed one important difference between the ATP-containing and
ATP-depleted mitochondria. In the presence of matrix ATP, both
pb2-(1-76)-DHFR (Fig. 2, upper panel, lane 3) and pSu9-(1-112)-DHFR (Fig. 2,
lower panel, lane 9) were imported into the
mitochondrial matrix, as they were largely protease-protected in
mitoplasts. In ATP-depleted mitochondria, efficient translocation
across the outer membrane occurred, but both proteins became arrested
in the inner membrane during import in an
Nin-Cout topology. This is demonstrated by MPP
processing of the N-terminal presequence and accessibility of the
C-terminal DHFR domain to added protease in mitoplasts (Fig. 2,
upper panel, lane 6; and lower panel,
lane 12). Therefore, their import into the matrix was
arrested at the level of the inner membrane in the absence of matrix
ATP, indicating lack of functional mt-hsp70. In the case of the other
cytochrome b2-derived preproteins, an Nin-Cout topology was achieved following import
into both matrix ATP-containing and ATP-depleted mitochondria. Thus,
the sorting process appears to proceed in a manner independent of
functional mt-hsp70 (Fig. 2, upper panel). The DHFR moiety
following import of each of the preproteins analyzed was folded,
irrespective of whether import into matrix ATP-containing or
ATP-depleted mitochondria was performed (data not shown).
In summary, preproteins of both intermembrane space- and matrix-targeted proteins bearing an N-terminal hydrophobic segment can be imported into mitochondria and become stabilized as translocation intermediates without requiring the activity of mt-hsp70. Stabilization in this manner appears to mediate the completion of translocation across the outer membrane in the absence of further mt-hsp70-driven import across the inner membrane. Import in this mt-hsp70-independent manner occurs not only for intermembrane space-targeted proteins, but also as efficiently for a matrix-targeted protein bearing a hydrophobic insertion signal. In contrast, hydrophilic matrix-targeted proteins cannot be stabilized as translocation intermediates in the absence of mt-hsp70 binding, and hence, their import displays an absolute dependence on mt-hsp70 action.
Differential Requirement for mt-hsp70 in Preventing Retrograde Movement of Translocation IntermediatesWe asked whether the
hydrophobic segment in a preprotein is sufficient to prevent retrograde
translocation of methotrexate-arrested intermediates when stalled at
the level of the inner membrane following the release of bound
mt-hsp70. Retrograde translocation of methotrexate-arrested preproteins
was analyzed in both mitochondria and mitoplasts (Fig.
3). pb2-(1-76)-DHFR,
pb2-(1-85)-DHFR, and pb2-(1-109)-DHFR were imported into either
wild-type mitochondria or mitoplasts in the presence of methotrexate,
where they became arrested as translocation intermediates, processed by
MPP in the matrix (Fig. 3). These translocation intermediates were
associated with the import sites in a stable manner when further
incubated in the presence of ATP and a membrane potential. Depletion of the matrix ATP results in the release of bound mt-hsp70 from the translocating polypeptide chain (15). Under these conditions, the
MPP-processed forms of pb2-(1-76)-DHFR and
pb2-(1-85)-DHFR underwent retrograde
translocation and were released from the mitochondria into the
supernatant (Fig. 3, +Oli/Ap). Dissipation of the membrane
potential by addition of valinomycin led also to a release of the
methotrexate-arrested intermediates (Fig. 3, +Val). In
contrast, the MPP-processed form of
pb2-(1-109)-DHFR remained associated with the
mitochondria under both of these conditions, suggesting that it had
become stabilized in a manner no longer dependent on and
mt-hsp70 binding. When accumulated in mitoplasts, all preproteins
remained tightly associated as translocation intermediates, even under
conditions of matrix ATP depletion and
dissipation (Fig. 3,
hatched bars). A control hydrophilic matrix-targeted
protein, pSu9-(1-69)-DHFR, when arrested with methotrexate in
mitoplasts and mitochondria, underwent retrograde translocation upon
both of these treatments (data not shown) (12).
In conclusion, penetration of the hydrophobic segment to the translocase of the inner membrane leads to maintenance in the import channel and prevention of retrograde translocation upon release of bound mt-hsp70. The common denominator for mt-hsp70-independent stabilization appears to be the interaction of a suitably positioned hydrophobic core with component(s) of the TIM channel, rather than a particular recognition of a sorting signal specific for one mitochondrial sublocation or another.
Matrix ATP Requirement for the Stabilization of Cytochrome b2 Bearing a Mutation in the Sorting SignalTo
investigate the specificity of the sorting signal in more detail, we
analyzed the import of a cytochrome b2
derivative, pb2RIC-(1-167)-DHFR,
which bears mutations in the essential cluster of positively charged
amino acids (Arg-Lys-Arg) just prior to the hydrophobic core of the
sorting signal. This mutated preprotein becomes missorted to the matrix
in an ATP/mt-hsp70-dependent manner. In the absence of
functional mt-hsp70, it is imported into the intermembrane space, where
it is matured by the Imp1p protease (18). In the presence of matrix
ATP, pb2RIC-(1-167)-DHFR was
rapidly imported into the mitochondria (Fig. 4), where
it was localized to the matrix (data not shown). The decrease in the
signal at later time points reflected degradation of the
matrix-accumulated species by the Pim1p protease, as reported previously (31). In ATP-depleted mitochondria,
pb2RIC-(1-167)-DHFR was imported
with reduced kinetics (Fig. 4), and it accumulated in the intermembrane
space (data not shown) (18). On the other hand, wild-type
pb2-(1-167)-DHFR was largely unaffected by
alterations in the matrix ATP levels (Fig. 4). Despite the mutation in
the sorting signal,
pb2RIC-(1-167)-DHFR could be as
effectively imported into the mitochondria as its wild-type counterpart
in the absence of functional mt-hsp70. We conclude therefore that the
mt-hsp70-independent stabilization observed is not dependent on a
functional sorting signal, but rather on the presence of an intact
hydrophobic core.
Import Intermediates of pSu9-(1-112)-DHFR Remain in the TIM Machinery in the Absence of mt-hsp70 Binding
Do preproteins
stabilized in an mt-hsp70-independent manner remain in the environment
of the TIM machinery? In a first approach, pSu9-(1-112)-DHFR was
arrested as a translocation intermediate in mitoplasts by import in the
presence of methotrexate. Cross-linking to TIM17, TIM44, and mt-hsp70
was observed (Fig. 5A, +ATP).
Following arrest, the matrix ATP levels were reduced by an
oligomycin/apyrase treatment as described previously (15). The
translocation intermediate was still found in the environment of
components of the TIM machinery, as it could be cross-linked to TIM44
and TIM17, whereas the mt-hsp70-cross-linked adduct was missing
(Fig. 5A, ATP).
In a second approach, pSu9-(1-112)-DHFR was imported into matrix
ATP-depleted mitochondria, where it accumulated in the intermembrane space spanning the inner membrane (Fig. 5B,
chase). Upon replenishment of matrix ATP levels, this
accumulated species could be further chased across the inner membrane
into the matrix (Fig. 5B, +chase). In conclusion,
the arrested translocation intermediate in ATP-depleted mitochondria
remains a productive one, associated with an active TIM machinery
through its hydrophobic segment.
The import of mitochondrial preproteins containing N-terminal hydrophobic segments does not depend on an early interaction with mt-hsp70. As we show here, this is in contrast to the import of hydrophilic proteins. By virtue of such hydrophobic segments, preproteins become stabilized in the TIM machinery. This occurs apparently by interaction with component(s) that either are part of the TIM channel or are in close proximity to the TIM channel. Stabilization in this manner can lead to processing by MPP in the matrix and completion of passage over the outer membrane.
This observation sheds light on a number of aspects of mitochondrial protein import and sorting. First, import and stabilization in this manner are not unique to sorting signals that normally direct the preprotein to the intermembrane space, such as the cytochrome b2 signal. Rather, matrix-targeted proteins containing hydrophobic segments (such as subunit 9 of the F1F0-ATPase and nonfunctional cytochrome b2 sorting signals retaining intact hydrophobic cores) are also stabilized with equal efficiencies. A similar observation was made with cytochrome c1-derived sorting signal mutants.2 Apparently, the hydrophobicity of a sorting signal, rather than its specificity for a particular sorting pathway, is responsible for the phenomenon of mt-hsp70-independent stabilization and import. Hence, the observed mt-hsp70 independence of import is not a characteristic of preproteins sorted to the intermembrane space, although it has been repeatedly taken as support for a "stop-transfer"-type mechanism.
Second, the hydrophobic segments must penetrate into the inner membrane to stabilize the translocating polypeptide chain in the import channel in a membrane potential- and an mt-hsp70-independent manner. If the sorting signal is physically restricted from reaching as far as the inner membrane (e.g. by a folded DHFR moiety), both the presence of a membrane potential and binding of mt-hsp70 to the incoming polypeptide are necessary for the prevention of retrograde translocation. The mt-hsp70-independent stabilization may be exerted by an interaction of the hydrophobic core with components of the TIM machinery in the inner membrane or by unknown components in the mitochondrial matrix.
Third, the position of the hydrophobic core relative to the presequence is critical for a preprotein to become stabilized in an mt-hsp70-independent manner. From results presented here and from the analysis of other inner membrane proteins such as cytochrome oxidase subunit Va and Sco1p (13, 32),3 it appears that a maximum distance of ~75 amino acids from the N terminus of the preprotein to its hydrophobic core can be tolerated if mt-hsp70-independent stabilization is to be ensured. In the case of cytochrome oxidase subunit Va, where the hydrophobic segment is ~100 amino acid residues from the N terminus, import is dependent on mt-hsp70 activity (13, 32); moving the hydrophobic sorting signal of cytochrome oxidase subunit Va closer to the N terminus conferred mt-hsp70 independence on the import process (32).
These findings support the following mechanism of protein transport across the inner membrane. Translocation of polypeptides can occur, at least of the N-terminal ~75 amino acid residues, by random reversible diffusion (33); mt-hsp70, by binding to preproteins upon their emergence in the matrix, then acts to shift the equilibrium to the trans-side of the inner membrane. The free diffusion across the inner membrane of these N-terminal regions would not support an import model where mt-hsp70 functions solely in a manner whereby it pulls segments of the polypeptide chain into the matrix (34, 35).
Our data suggest that matrix-targeted proteins containing a suitably positioned hydrophobic segment can artificially become arrested in the inner membrane. Is such a hydrophobic arrest mechanism used by at least a subset of inner membrane proteins, such as cytochrome oxidase subunit Va, as a physiological targeting pathway? Sorting by hydrophobic arrest most likely exists for some inner membrane proteins. We speculate that the TIM channel, perhaps together with other protein components of the inner membrane, scans the incoming polypeptide for the presence of hydrophobic cores. Recognition of such an element would result in a slowdown in translocation of the preprotein. Such a translocational arrest is necessary if the sorting signal is to laterally insert into the inner membrane. Hydrophilic sequences flanking the hydrophobic core appear to play an important role in the specificity of the process of lateral integration into the inner membrane.4 If such a lateral sorting signal is not present, translocation will proceed, resulting in matrix import of the hydrophobic core. This further translocation requires active mt-hsp70. If absent, the affinity of component(s) of the TIM channel for such a hydrophobic core is sufficient to trap the incoming polypeptide in the import channel. Under these conditions, complete translocation across the outer membrane can occur, but import across the inner membrane is blocked.
Is this arrest mechanism used by the cytochrome b2-derived proteins? The rates and efficiencies of import of these preproteins were found not to be adversely affected by the lack of mt-hsp70 activity. These data suggest that the cytochrome b2-derived preproteins follow the same sorting route irrespective of whether mt-hsp70 is functional or not. Only in the case of those cytochrome b2-derived proteins bearing an intact folded heme domain is their import dependent on mt-hsp70 intervention (28, 36, 37). We propose that the sorting signal enters the matrix, where it is specifically recognized and secured by a putative sorting signal recognition protein. The translocating preprotein then disengages from further involvement of the mt-hsp70 system for subsequent import. Evidence in favor of passage of at least N-terminal parts of mature-size cytochrome b2 through the matrix was recently presented; these sorting intermediates looped through the matrix while remaining in contact with components of the TIM machinery (21).
We thank Sandra Weinzierl for excellent technical assistance and Dr. Thomas Langer for helpful discussions.