(Received for publication, March 3, 1997, and in revised form, April 1, 1997)
From the Unité de Biochimie Physiologique,
Université catholique de Louvain, Place Croix du Sud, 2-20, B-1348 Louvain-la-Neuve, Belgium, and the ¶ Botanisches Institut
der Universität zu Köln, Gyrhofstrasse 15, D-50931
Köln, Germany
The triose phosphate 3-phosphoglycerate phosphate translocator (TPT) is a chloroplast envelope inner membrane protein whose transit peptide has structural properties typical of a mitochondrial presequence. To study the TPT transit peptide in more detail, we constructed two chimeric genes encompassing the TPT transit peptide and either 5 or 23 amino-terminal residues of the mature TPT, both linked to the reporter chloramphenicol acetyltransferase (cat) gene. The precursors were synthesized in vitro and translocated to and processed in purified plant mitochondria. However, this import was not specific since both precursors were also imported into isolated chloroplasts. To extend this analysis in vivo, the chimeric genes were introduced into tobacco by genetic transformation. Analysis of CAT distribution in subcellular fractions of transgenic plants did not confirm the data obtained in vitro. With the construct retaining only 5 residues of the mature TPT, CAT was found in the cytosolic fraction. Extension of the TPT transit peptide to 23 residues of the mature TPT allowed specific import and processing of CAT into chloroplasts. These results indicate that, despite its unusual structure, the TPT transit peptide is able to target a passenger protein specifically into chloroplasts, provided that NH2-terminal residues of the mature TPT are still present. The discrepancy between the in vitro and in vivo data suggests that the translocation machinery is more stringent in the latter case and that sorting of proteins might not be addressed adequately by in vitro experiments.
Mitochondria and chloroplasts have their own genetic information. However, these endosymbionte-derived genomes have a limited coding capacity, as most of their genes were transferred to the nucleus during evolution. The majority of the organellar proteins are thus nuclear-encoded and synthesized in the cytosol as larger precursor forms. The latter usually have an amino-terminal targeting sequence (called presequence for the mitochondria and transit peptide for the chloroplast), which is responsible for directing transport of the precursors to their respective organelles (1-3).
The mitochondrial and chloroplast targeting signals have some
intriguing structural similarities. Both are rich in basic and hydroxylated amino acids and usually lack acid and apolar amino acid
residues (4, 5). However, their predicted secondary structures differ.
Whereas mitochondrial presequences are predicted to form an amphiphilic
-helix, chloroplast transit peptides display a random coil structure
(6, 7). As a consequence, the in vivo import process is
assumed to be specific to each organelle. This has been observed
experimentally (2, 8-10), indicating that protein import into
mitochondria and chloroplasts follows different routes.
An unusual situation is observed with the chloroplast triose phosphate
3-phosphoglycerate-phosphate translocator
(TPT),1 a protein of the chloroplast
envelope inner membrane. This transporter is encoded in the nucleus and
synthesized as a higher molecular weight precursor in the cytosol. It
bears an NH2-terminal transit peptide, which is assumed to
direct transport across the envelope membrane (11). Recently it was
shown by in vitro import studies that the transit sequence
contains only stromal targeting information and that a hydrophobic
region of the NH2-terminal of the mature TPT might be
responsible for directing the protein to the inner envelope membrane
(12, 13). Several phosphate translocator genes have been isolated from
various species. Analysis of the structures predicted for the various
transit peptides reveals, in the majority of cases, the presence of a
positively charged amphiphilic -helix in the
NH2-terminal region (14, 15). Interestingly, this feature
is typical of mitochondrial presequences. Consistent with this
observation is the report that the phosphate translocator is imported
and processed in mitochondria isolated from yeast and broad bean (16).
However, these data did not prove that the TPT transit peptide was
sufficient for in vitro mitochondrial uptake. Moreover, the
hydrophobic nature of TPT made its analysis more difficult as, in
in vitro uptake assays, the mitochondrial outer membrane is
the only hydrophobic environment offered to the TPT precursor. The
paradox is thus that the TPT is imported in vitro both in
chloroplasts and in mitochondria, but that, in vivo, the TPT
localization is the chloroplast only. This suggests that in
vivo either TPT is only targeted to chloroplasts or that it is
targeted to both organelles and destroyed in mitochondria. To resolve
this conflict, we prepared two chimeric genes linking the TPT
translocator transit peptide and either 5 or 23 residues of the
NH2-terminal mature protein, to chloramphenicol
acetyltransferase (CAT), a soluble reporter protein. We show here that
the TPT transit peptide can direct transport of CAT into both isolated
chloroplasts and mitochondria. However, when the same constructs were
tested in transgenic plants, CAT was found mainly in the cytosol or in the chloroplast depending on whether the TPT transit peptide was followed by 5 or 23 residues of the mature TPT. These results question
the in vitro approach to studying specificity of targeting. They also indicate that the TPT transit peptide requires residues of
the amino part of the mature TPT for specific in vivo
targeting to the chloroplast.
Standard procedures were used for DNA
manipulations (17). The constructs assembling the TPT transit peptide
and CAT were made as follows. The pSP72 plasmid carries a cDNA
fragment corresponding to the 5-noncoding region, the entire transit
peptide, and 42 amino acids from the mature spinach phosphate
translocator (11). This fragment was released by HindIII and
BglII digestion. Two 3
-shortened fragments were obtained by
polymerase chain reaction. The first fragment (TPT5) corresponds to the
entire TPT transit peptide and 5 amino acids from mature TPT; the
second (TPT23) comprises the whole TPT transit peptide and 23 amino
acids from mature TPT. Synthetic primers provided with flanking
HindIII sites were as follows.
The TPT5 and TPT23 upstream primer was 5-
CCCCCAACTTCTTCCGACAATGGAG.
The TPT5 downstream primer was
5-CCCCCAAGCTTCCAGAGCCACTAGCGGC.
The TPT23 downstream primer was
5-CCCCCAAGCTTCCGCCAGTGACAAGAGC.
After polymerase chain reaction amplification, the fragments were digested with HindIII and cloned into the HindIII site of the polylinker region of SK(+) Bluescript (Stratagene), resulting in the TPT5 and TPT23 plasmids, respectively. Both constructs were sequenced.
The CAT encoding sequence was isolated by HindIII and
BamHI digestion of plasmid pBin35ScatE9 (18) and inserted
into the corresponding sites of SK(+) Bluescript, resulting in the CAT plasmid. The HindIII site previously used for inserting
targeting sequences (8, 18) is localized 75 nucleotides upstream of the
CAT translation initiation codon. When translated, this region encodes
a cryptic mitochondrial cleavage site (18). Using polymerase chain
reaction, therefore, we engineered a new CAT gene provided with a
HindIII site 10 nucleotides upstream of the CAT translation initiation codon. Primers were as follows.
The upstream primer was 5-CCCCCAAGCTTGGAAGCTAAAATGGAG.
The downstream primer was 5-CCATACGGAATTCCGG.
This new construct was checked by sequencing.
To prepare the TPT-CAT constructs, the TPT5 and TPT23 fragments were obtained by HindIII digestion and cloned at the HindIII site of the modified CAT plasmid digested previously with HindIII, resulting in TPT5-CAT and TPT23-CAT.
TPT-CAT constructs for tobacco transformation were prepared as follows.
The TPT5-CAT and TPT23-CAT plasmids were digested with BamHI
and partial HindIII, releasing the fragments TPT5-CAT and
TPT23-CAT. These fragments were inserted into the corresponding sites
of Bin35ScatE9 (18), digested previously with HindIII and
BamHI, producing the plant transformation vectors
Bin35S-TPT5-CAT and Bin35S-TPT23-CAT, respectively.
The plasmids TPT5-CAT and TPT23-CAT were linearized with BamHI. Transcription was carried out in the presence of 7mGpppG using T7 RNA polymerase (19). Translation was performed in a reticulocyte lysate system (Boehringer Mannhein) in the presence of [35S]methionine (Amersham).
In Organello ImportIn vitro import reactions were performed with broad bean mitochondria isolated from dark-grown hypocotyls as described previously (19), except that 1% bovine serum albumin was added to the import medium. In vitro import in spinach chloroplasts was performed as described by Bartlett et al. (20).
Plant TransformationPlant expression vectors were mobilized in the Agrobacterium tumefaciens strain LBA 4404 by triparental mating. Helper plasmid pRK 2013 (21) was used. Leaf discs of Nicotiana tabacum cv SR1 were infected, and transgenic plants were raised as described (22). All the experiments reported here were carried out on F1 plants obtained after self-crossing.
Fractionation of Tobacco Cells and Protein QuantitationSubcellular fractions were obtained from 10 g of leaves as described previously (18), except that homogenization was performed in 50 ml of homogenization buffer and that 0.2% (w/v) polyvinylpyrrolidone was added to the buffer.
Purification of chloroplasts and thykaloids on a continuous Percoll gradient was performed as described (23).
Protein concentration was determined by the enhanced alkaline copper assay (24) using bovine serum albumin as a standard.
Western Blot AnalysisAfter sodium dodecyl
sulfate-polyacrylamide gel electrophoresis, proteins were transferred
to a nitrocellulose membrane and immunodetected with antibodies raised
against purified CAT (1/1,000), lipoamide dehydrogenase (1/8,000),
ribulose 1,5-bisphosphate carboxylase (1/20,000) followed by
125I-protein A (see Fig. 4, A and C
and Fig. 5) or chemiluminescence (see Fig. 4B) detection.
Signals were quantitated using an Image Master densitometer (Pharmacia
Biotech Inc.).
The TPT has been shown to be imported in
vitro into isolated chloroplasts (11). We replaced the mature TPT
by the CAT reporter protein for a double purpose. First, it exchanged a
hydrophobic protein for a soluble passenger protein and therefore
avoided the problem of unspecific binding of the precursor to the outer chloroplast or mitochondrial membrane through hydrophobic interactions. Second, it enabled us to test directly the ability of the transit peptide on its own to target a protein to either chloroplasts or
mitochondria. CAT was chosen because it had previously been shown to be
targeted to either organelle according to the targeting sequence (8).
Two constructs were prepared (Fig. 1). One, TPT5-CAT, retained 5 residues of the mature TPT to still allow cleavage of the
transit peptide which might have required surrounding residues. The
second construct, TPT23-CAT, included 23 residues of the mature TPT, in
case the amino-terminal part of the mature TPT was also involved in
targeting, as this had already been shown for the chlorophyll
a/b-binding protein (25, 26).
Both chimeric genes were placed on an Escherichia coli
plasmid, under the control of the T7 RNA polymerase promoter. RNA
transcribed in vitro was translated in a rabbit reticulocyte
lysate in the presence of [35S]methionine. The precursors
(Fig. 2, lanes 1 and 6) were
imported into spinach chloroplasts and processed to a mature protein
(lanes 2 and 7), whose size, compared with that
of CAT without a transit sequence (lane 5), was compatible
with the extra 11 (TPT5-CAT) or 29 (TPT23-CAT) residues remaining
upstream of the CAT initiation codon (Fig. 1). The mature CAT was
inside the chloroplast, as a brief sonication released it into the
soluble fraction (lanes 3 and 8). We therefore
concluded that the TPT transit peptide with 5 or 23 residues of the
mature protein was sufficient to target a foreign protein in
vitro into chloroplasts. No further analysis was performed with
chloroplast import as our results were in agreement with the data
showing that the TPT transit peptide is a signal for in
vitro stromal targeting (12, 13).
The TPT Transit Peptide Addresses a Reporter Protein into Isolated Mitochondria
The spinach TPT precursor has been shown to be
imported in vitro into plant or yeast mitochondria (16).
In vitro mitochondrial uptake of the TPT-CAT precursors was
therefore performed with mitochondria isolated from etiolated seedlings
of broad bean. This material, which circumvents the problem of
contaminating chloroplasts, was shown previously to allow the uptake of
mitochondrial, and not chloroplast, precursors (19). Incubation of the
labeled precursors (Fig. 3A, lanes
2 and 6) with purified mitochondria produced a cleaved
mature form (lanes 3 and 7), whose size, compared with that of CAT without the additional sequence (lanes 1 and 5), suggests that cleavage occurred between the transit
peptide and the sequence kept from the mature TPT (Fig. 1). The mature proteins were protected against externally added proteinase K, indicating that they were effectively imported into the organelle (Fig.
3A, lanes 4 and 8). Contrary to the
import experiment performed with chloroplasts (Fig. 2), a significant
amount of unprocessed precursor was found bound to the mitochondria but
was degraded upon proteinase K digestion. A similar observation has
been reported for a truly mitochondrial precursor (19).
As 5TPT-CAT and 23TPT-CAT behaved similarly, the next experiments were performed using the shortest construct only. To show the dependence of TPT5-CAT mitochondrial uptake on import machinery, we performed in vitro uptake experiments in the presence of valinomycin, a potassium ionophore and an uncoupler of oxidative phosphorylation (Fig. 3B). Mitochondrial import of TPT5-CAT was prevented (lanes 4 and 5), indicating that uptake depends on an electrochemical potential across the inner mitochondrial membrane. Import was also prevented when oligomycin, a specific inhibitor of the mitochondrial ATP synthase, was added to the import medium (Fig. 3B, lanes 6 and 7). Import thus requires internal ATP. Other import parameters were found to be typical of mitochondrial import: requirement of external ATP, absence of import at 0 °C or with trypsin-treated mitochondria (data not shown). In conclusion, properties of the in vitro import of TPT-CAT precursors into mitochondria are similar to those of the import of a truly mitochondrial protein.
In Vivo Targeting Properties of the TPT Transit PeptideThe
results reported so far support the conclusion that the TPT transit
peptide is capable of addressing a passenger protein in
vitro into both isolated chloroplast and mitochondria. Moreover, this import displays the expected properties of a process that depends
on a functional translocation machinery. Since TPT has never been found
in vivo in plant mitochondria, it could be hypothesized that
sequences within the mature TPT and absent in the chimeric proteins
analyzed here are involved in specifically directing the protein to
chloroplasts. An alternative explanation would be to consider that
in vitro uptake does not reflect what occurs in
vivo, possibly due to a lack of the cytosolic factors involved in
targeting specificity. Finally, we also have to consider the possibility that in vivo TPT is also targeted to
mitochondria but rapidly degraded. To evaluate these hypotheses, we
equipped the TPT5-CAT and TPT23-CAT constructs with the 35S
transcription promoter of cauliflower mosaic virus and the 3-noncoding
region of a pea Rubisco small subunit gene. The chimeric genes were
introduced into tobacco, using an A. tumefaciens Ti
plasmid-derived vector. Transgenic plants were selfed, and several
independent F1 plants were characterized for both constructs.
Subcellular fractionation of the plant material was performed by centrifugation to obtain a crude cytosolic supernatant and a crude organellar pellet. Chloroplast- and mitochondria-enriched fractions were also obtained by differential centrifugation and subsequent purification of the organelles on Percoll gradients. To evaluate organelle enrichment, we immunodetected in the various fractions the large subunit of Rubisco, a soluble marker of the chloroplastic stroma, and the lipoamide dehydrogenase, a soluble mitochondrial marker found in several mitochondrial matrix enzymes (27). Distribution of these markers among the various fractions was analyzed by Western blot (an example is shown in Fig. 4A) and quantitated by image analysis (Fig. 4C). The majority of the Rubisco was released into the supernatant, confirming the high sensitivity of tobacco chloroplasts to mechanical grinding (26). Enrichment in the chloroplast fraction was low, but this has to be expected since chloroplast proteins of mesophyll cells represent up to 50% of total proteins and the highest enrichment can therefore be only 2-fold. In contrast, the majority of the mitochondrial marker was found in the crude organellar pellet and was enriched about 10-fold in the mitochondrial fraction. A certain amount of Rubisco was found in the mitochondria-enriched fraction. As discussed previously (26), it is not clear whether this stems from the presence of intact chloroplasts in the mitochondria-enriched fraction or from the binding to mitochondria of Rubisco released during grinding.
Western blot (or enzyme activity, not shown) analysis of CAT in a TPT23-CAT plant shows that the reporter protein was addressed to chloroplasts since CAT and Rubisco enrichment in the chloroplast fraction was similar (Fig. 4A). There was no enrichment in the mitochondrial fraction. As expected, the size of the mature CAT observed for TPT23-CAT in the chloroplast fraction (Fig. 4B) was larger than that of a control cytosolic CAT without any targeting sequence. This difference accounts for the 23 residues of mature TPT and 6 residues from the linker region.
Quantification of Western blot data from independent TPT23-CAT transgenic plants confirmed the presence of CAT within the chloroplast (Fig. 4C). However, we observed that CAT enrichment in the crude organellar fraction was higher than enrichment of Rubisco in the same fraction, suggesting that the processed TPT23-CAT somehow binds to chloroplast membranes in vivo or after homogenization. To analyze this point, we centrifuged a chloroplast fraction on a self-generated Percoll gradient. As expected, two main green bands were obtained, corresponding to the intact chloroplasts (heavier band) and thykaloids (lighter band). This was confirmed by gel electrophoresis analysis (Fig. 5), showing in fraction 3, the heaviest green peak, the bands corresponding to the large subunit of Rubisco and the chlorophyll a/b-binding protein, the two major soluble and membrane chloroplast proteins, respectively. Fraction 7, the other green peak, still contains the chlorophyll a/b-binding protein but not Rubisco, confirming that it corresponds to thykaloids. CAT was found to peak with intact chloroplasts (fraction 3), thykaloids (fraction 8), and a top fraction (11) where bovine serum albumin (67 kDa) could be detected, thus corresponding to the soluble fraction. These observations therefore suggest that part of the CAT within the TPT23-CAT plant is in the chloroplast stroma, and part binds to the thykaloids. This was confirmed by showing the sensitivity of CAT to thermolysin in the thykaloid and soluble fractions but not in the intact chloroplast fraction (data not shown).
For the TPT5-CAT plant, however, CAT remained essentially in the supernatant (Fig. 4, A and C). Little, if any, activity was found in the chloroplast or mitochondrial fractions. We therefore conclude that in vivo the TPT transit peptide together with 5 residues of the mature TPT is not sufficient to address CAT into chloroplasts.
The size of CAT within the TPT5-CAT plant was found to be similar to that of control cytosolic CAT (Fig. 4B), suggesting that TPT5-CAT was nevertheless processed in the cell by some kind of cytosolic proteolytic activity or, after homogenization, by a protease released from an organelle. Homogenization of the plant material in the presence of phenol gave similar results (data not shown), suggesting that processing probably occurs in vivo. To exclude any DNA rearrangement during A. tumefaciens or plant transformation which could have removed the TPT transit peptide initiation codon, we used polymerase chain reaction to retrieve a DNA fragment encompassing the NH2-terminal region of TPT5-CAT from a TPT5-CAT-transformed plant. We then checked by sequencing that the sequence was not modified.
TPT is a chloroplast protein and has never been detected in
mitochondria. Consistent with this is the observation that the TPT
precursor is addressed to, and processed in, isolated chloroplasts (11). Recent reports (12, 13) showed that the TPT transit peptide
serves in vitro as a targeting signal to the chloroplast stroma. Here we showed that the TPT transit peptide is able to address
a foreign protein to chloroplasts. The TPT precursor, however, is also
imported in vitro into mitochondria isolated from yeast and
plants, and this process has shown the typical features of specific
protein import such as energy requirement and protease-sensitive
binding of the precursor to the yeast MOM19 receptor (16). The data
reported here with two precursors retaining the transit peptide and 5 or 23 residues of mature TPT delimit the sequence involved in in
vitro mitochondrial targeting within a region spanning the 80 residues of the transit peptide and the 5 NH2-terminal
residues of the mature TPT. This transport requires a membrane
potential and external ATP. These observations strongly suggest that
the mitochondrial import of the TPT-CAT precursors occurs via a normal
import route. Examination of the primary structure of the TPT transit
peptide from various sources suggests the presence of a putative
positively charged amphiphilic -helix (14, 15). This feature has
been shown to be important for membrane insertion and for the
translocation of imported mitochondrial precursors (4) and could
account for the TPT-CAT mitochondrial import.
In both in vitro chloroplast and mitochondrial import, the apparent size of the mature TPT5-CAT and TPT23-CAT is compatible with processing of the precursors at the expected cleavage site. As suggested previously (16, 26), this implies that proteases recognizing the same target are present in both mitochondria and chloroplasts.
A major conclusion of the data reported here is that the TPT transit peptide behaves differently in vitro and in vivo. In the latter case, indeed, the shortest construct (TPT5-CAT) remained in the cytosol. It could be argued that the targeting peptide of TPT5-CAT is degraded rapidly by a cytosolic protease, therefore preventing chloroplast import. This is, however, unlikely since it would imply that the additional 18 internal residues of TPT23-CAT confer protease resistance in the cytosol but not in the chloroplast. Another hypothesis would be that the NH2-terminal region of TPT5-CAT is engaged in the chloroplast import machinery, processed within the stroma, and, because of a failure of complete translocation, released back into the cytosol. This hypothesis, however, is not in agreement with the observation that in vivo cleavage of TPT5-CAT does not occur at the expected site as observed after in vitro targeting (see Fig. 2) but probably at, or very close to, the CAT initiation codon (see Fig. 4B). Moreover, interfering sequences within the CAT reporter are unlikely to be present since this protein has been used previously as a passenger for either mitochondrial or chloroplast import (8, 26). A more likely hypothesis would be that structural features required for in vivo mitochondrial or chloroplast uptake are missing in the TPT transit peptide. Failure of import could occur due to lack of interaction of the precursor either with specific chaperones involved in organellar targeting (28) or with receptors at the organelle outer membrane. The precursor would then be processed by a cytosolic protease. Cleavage of a chloroplast or mitochondrial targeting peptide of a chimeric protein which was not imported either has been observed before (26, 29).
When the TPT transit peptide was followed by 23 residues of mature TPT,
CAT was efficiently targeted in vivo to chloroplasts but not
to mitochondria. Since CAT stably accumulates in mitochondria when
linked to a truly mitochondrial presequence (8), we can conclude that
in vivo the TPT transit peptide together with 23 residues of
the mature protein does not constitute an in vivo mitochondrial targeting sequence. This weakens the hypothesis that TPT
would also be addressed in vivo to mitochondria and then destroyed rapidly. The requirement of sequences within the mature TPT
for import is not unexpected in itself. Similarly, the transit peptide
of the chlorophyll a/b-binding protein was unable
to direct either CAT or the -glucuronidase reporter protein into
chloroplasts unless sequences of the mature protein (25) or surrogate
sequences (26) were present. The similarity between TPT and the
chlorophyll a/b-binding protein goes no further
since the latter has a classical transit peptide and has been shown
previously to be addressed under the same experimental conditions
in vitro to chloroplasts and not to mitochondria (19). The
nature of the additional residues required for in vivo
chloroplast import is not clear. The amino-terminal part of the mature
TPT is not well conserved in various species. We could thus hypothesize
that secondary, instead of primary, structures might be involved.
A last conclusion from this work is that, as far as sorting is
concerned, caution is necessary when analyzing in vitro
import data. For instance, we found similar rates of in
vitro mitochondrial import for TPT5-CAT or TPT23-CAT as for a
construct linking CAT to a truly mitochondrial presequence, that of the
mitochondrial ATPase subunit, and yet in vivo the latter
construct was imported efficiently into mitochondria (18).
What could the explanation be for the different observations in vivo and in vitro? Since in the latter case, the precursors are radioactively labeled, the number of precursor molecules that are targeted to mitochondria is probably small compared with the number of mitochondria present in the assay. On a quantitative basis, the process is probably not very efficient. In vivo, the targeting machinery is expected to be very efficient (to avoid the accumulation of precursors into the cytosol) and specific (to avoid mistargeting). Concerning this last point, it could be argued that the in vitro uptake experiments are not very stringent since there is no competition for various subcellular compartments. Performing in vitro import in the presence of both mitochondria and chloroplasts would address this point but would mean first finding conditions that are appropriate for both types of import. In vivo specificity might be achieved by the affinity of the various precursors for their respective receptors localized at the outer face of organelles. However, specificity might occur at an earlier step, since precursors may bind to cytosolic or membrane chaperones after, or even during, their translation (28, 30, 31). In the framework of this hypothesis, our data suggest that in vivo binding to chaperones and/or to chloroplast receptors requires, in addition to the transit peptide, residues of the mature TPT protein.
We thank Dr P. Weisbeek for the Rubisco antiserum and P. Gosselin for excellent technical assistance.