From the Department of Agricultural Botany, Faculty of Agriculture, Hebrew University of Jerusalem, Rehovot 76100, Israel
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ABSTRACT |
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The proteases involved in proteolytic degradation
in the thylakoid lumen are largely unknown. Western analysis with an
antibody against the Escherichia coli periplasmic serine
protease DegP suggested that pea chloroplasts contain a homologue of
this protease. This homologue was peripherally bound to the luminal
side of the thylakoid membrane and could only be removed by a
combination of high salt and non-ionic detergent. Its level increased
almost 2-fold in pea seedlings exposed to elevated temperature for
4 h, suggesting this protease's role in the chloroplast's heat
response. Isolated thylakoid membranes containing the chloroplastic
homologue of DegP degraded -casein, an in vitro
substrate of the bacterial protease. This activity was partially
inhibited by a serine protease inhibitor, suggesting that at least part
of the casein-degrading activity in the thylakoid membrane is
attributable to DegP. The existence of chloroplastic DegP was further
supported by isolating a full-length Arabidopsis cDNA
(designated AtDegP) encoding a protein that is 37%
identical and 60% similar to the E. coli protease. The
amino terminus of the deduced amino acid sequence contained a bipartite
transit peptide, typical of proteins targeted to the thylakoid lumen,
and the mature portion of the protein contained the highly conserved
serine protease catalytic triad His-Asp-Ser. The possible physiological
roles of chloroplastic DegP protease are discussed.
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INTRODUCTION |
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The chloroplast, the photosynthetic organelle of eukaryotic cells, is composed of six compartments: three different membranes and the three aqueous compartments delimited by them. The chloroplast envelope, composed of an outer membrane, an inner membrane, and an intramembrane space, surrounds the stroma, the soluble compartment where most carbon metabolism reactions take place. The third membrane is the extensive network of thylakoid membranes, harboring the photosynthetic antennae, the photosynthetic electron transport system, and the ATP synthesis machinery. The sixth compartment is the thylakoid lumen, into which protons are pumped to form a proton gradient across the thylakoid membrane. This gradient is the driving force for ATP synthesis. Proteins found within the lumen, either soluble or bound to the inner side of the thylakoid membrane, include the oxygen-evolving complex of photosystem II, components of the photosynthetic electron transport system, and many as yet unidentified proteins. As in other biological systems, maintenance of the lumen is expected to require protein degradation to remove damaged or otherwise nonfunctional proteins. However, the proteolytic machinery in this compartment has never been detailed.
Many examples of protein degradation in the chloroplast have been documented (for review, see Ref. 1). Specific degradation of luminal proteins has also been demonstrated, with plastocyanin being the best characterized example. When Chlamydomonas cells are grown in a Cu2+-deficient medium, apoplastocyanin is synthesized, imported into the chloroplast, and translocated across the thylakoid membrane; however, it fails to accumulate due to rapid degradation (2). A similar observation was made recently in an in vitro system. Apoplastocyanin was sensitive to proteolytic digestion, whereas the native or reconstituted holoproteins were not (3). This increased sensitivity of the apoprotein probably resulted from its lacking the characteristic secondary structure displayed by the holoprotein, as revealed by circular dichroism spectroscopy (3). In another recent study, truncated forms of a 23-kDa subunit of the oxygen-evolving complex, OE23, were correctly targeted to the lumen and processed to their mature size, but then rapidly degraded (4). These results suggest that the lumen contains its own proteolytic machinery, capable of degrading unassembled or damaged soluble proteins. It also implies that luminal proteases participate in the degradation of thylakoid membrane proteins exposed to the lumen.
Limited proteolytic processing also occurs in the lumen. Nuclear encoded thylakoid proteins, targeted to the lumen by N-terminal "thylakoid transfer" signals, are processed to their mature forms by a membrane-bound thylakoid-processing peptidase (5-7) that has not yet been purified or cloned. The plastid-encoded D1 protein of the photosystem II reaction center is also processed in the lumen. It is synthesized with a C-terminal extension of 8-16 amino acids that is removed within the thylakoid lumen immediately after synthesis (8, 9). Why this protein is synthesized with this extension is not clear, but its proteolytic removal is necessary to establish active photosystem II (10). The enzyme involved in this activity has been partially purified (8, 11) and characterized as a monomeric protein of 45 kDa (12). Recently, the gene encoding this peptidase was isolated from cyanobacteria (13) and spinach (14) and was found to be homologous to the periplasmic protease Tsp (tail-specific protease) of Escherichia coli, which is responsible for C-terminal processing of at least two bacterial proteins (13-16). Interestingly, it is also responsible for complete degradation of some proteins in E. coli (16). However, whether the luminal homologue of Tsp can also participate in complete degradation or, alternatively, its activity is limited to C-terminal processing of the D1 protein is unknown.
The occurrence of a homologue of the bacterial periplasmic protease Tsp in the lumen suggests the existence of other periplasmic protease homologues there. This idea is also supported by the notion that the lumen is functionally and evolutionarily equivalent to the bacterial periplasm. Both are compartments into which protons are pumped by the respective ATPases, and the machinery responsible for protein translocation into the lumen resembles that into the bacterial periplasm (7, 17).
To identify other homologues of bacterial periplasmic proteases in the
lumen, we initiated an immunological screening and data base search for
a chloroplastic homologue of the bacterial periplasmic serine-type
heat-shock protease DegP (also known as HtrA or Protease Do) (18-22).
A DegP homologue was found in the thylakoid, strongly associated with
the inner side of the thylakoid membrane. This suborganellar fraction
also exhibited the ATP-independent, serine-type -casein-degrading
activity typical of bacterial DegP. Moreover, expression of the
chloroplastic homologue was rapidly stimulated by high temperature.
Isolation of a cDNA encoding this protein and features of its
sequence support its localization and proposed activity.
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EXPERIMENTAL PROCEDURES |
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Plant Growth--
Pea seedlings (Pisum sativum var.
Alaska) were germinated and grown at 25 °C for 10-12 days under a
12-h photoperiod, at a light intensity of 150 microeinsteins·m2·s
1. To test the
effects of high temperature, seedlings were thoroughly watered and then
transferred to an incubator kept at 40 °C.
Chloroplast Isolation and Fractionation-- Intact chloroplasts were purified on Percoll gradients (23). They were subfractionated by osmotic shock in 10 mM Hepes, pH 8.0, followed by a 10-min centrifugation in an Eppendorf centrifuge at 4 °C. The supernatant, containing stromal extract, was separated from the pellet containing intact thylakoids; the latter was then washed twice and resuspended in 110 mM sorbitol and 17 mM Hepes-KOH, pH 8.0, to 2 mg of chlorophyll/ml. Intact thylakoids were further fractionated by sonication on ice, three times for 10 s each, with 1-min cooling intervals. The sonicated thylakoids were then centrifuged for 5 min in an Eppendorf centrifuge at 4 °C to remove intact thylakoids, and thylakoid membranes were separated from the lumen extract by ultracentrifugation of the supernatant at 200,000 × g for 1 h. The pellet containing thylakoid membranes was resuspended in 10 mM Hepes-KOH, pH 8.0, to 2 mg of chlorophyll/ml.
Intact Thylakoid and Thylakoid Membrane Treatments-- Intact thylakoids, as well as thylakoid membranes, were incubated in 0.1 mg/ml thermolysin on ice for 15 min. The reaction was terminated by adding a 5 mM EDTA. Intact thylakoids were then collected by a 5-min centrifugation in an Eppendorf centrifuge at 4 °C; washed once in 10 mM Hepes-KOH, pH 8.0; and resuspended in the same medium. Thylakoid membranes were collected by ultracentrifugation at 200,000 × g for 30 min. Intact thylakoids and thylakoid membranes were finally resuspended in 10 mM Hepes-KOH, pH 8.0, to a concentration of 1 mg of chlorophyll/ml.
To characterize the association between the proteins and thylakoid membranes, they were washed in high salt and/or low detergent concentrations. The membranes were resuspended in 1 M NaBr, 1 M NaCl, or 1 M NaCl supplemented with 0.05% Triton X-100 and incubated on ice for 30 min prior to ultracentrifugation at 200,000 × g for 30 min. The pellets were resuspended in 10 mM Hepes-KOH, pH 8.0, to a concentration of 1 mg of chlorophyll/ml.Polyacrylamide Gel Electrophoresis and Immunoblot Analysis-- Proteins were resolved on polyacrylamide gels (23) and blotted onto nitrocellulose membranes. DegP was detected with an antibody against the E. coli protein (18), generously donated by B. Lipinska (University of Gdansk, Gdansk, Poland). This antibody was used at a 1:100 dilution. Antibodies against the luminal 33-kDa subunit of the oxygen-evolving complex, OE33 (donated by N. Hoffman, Carnegie Institution), were used at a dilution of 1:10,000. Samples contained 7 and 0.1 µg of chlorophyll/lane (or their equivalent for stroma and lumen samples) for detection of DegP and OE33, respectively. Antigen-antibody complexes were visualized by enhanced chemiluminescence (ECL), and bands were quantified by laser densitometry.
Casein Degradation Assay--
Casein-degrading activity was
determined using a method previously described to assay bacterial DegP
activity (18). Reaction mixtures for the proteolytic activity assay
contained 0.3 mg/ml -casein (Sigma), 0.4 mg of chlorophyll/ml of
thylakoid membranes, and 50 mM Tris-HCl, pH 6.8, and the
reaction was carried out at 37 °C. Where indicated, 1 mM
phenylmethylsulfonyl fluoride and 4 mM
o-phenanthroline were included in the reaction mixture.
Proteins were then resolved by SDS-polyacrylamide gel electrophoresis
on 15% acrylamide gels, and the relative amount of casein in each sample was quantified by laser densitometric scanning of the Coomassie Blue-stained gel.
Cloning and Sequencing of AtDegP
cDNA--
Arabidopsis expressed sequence tag 125C11T7
showing homology to E. coli DegP and the
Arabidopsis cDNA library -PRL2 were obtained from the
Arabidopsis Biological Resource Center at Ohio State
University. A 680-base pair XbaI fragment was isolated from the expressed sequence tag clone, radioactively labeled, and used as a
DNA probe to screen the cDNA library. Isolated phages were excised
in vivo, plasmid DNA was prepared, and the longest clones were further analyzed. Automated sequencing of both strands was performed in an Applied Biosystems Model 373 DNA Sequencer. DNA and
deduced amino acid sequences were analyzed with the Genetics Computer
Group program.
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RESULTS |
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Thylakoid Membranes Contain a Homologue of DegP Protease-- On preliminary immunoblots of pea chloroplasts with an antibody against bacterial DegP, we detected a single band with apparent molecular mass of ~40 kDa (Fig. 1A), suggesting that this protease has a homologue in chloroplasts. When chloroplasts were fractionated, the cross-reacting protein was detected in the intact thylakoid fraction, protected from external protease treatment (Fig. 1B). Similar results were obtained using an antibody against OE33, localizing chloroplastic DegP to within the thylakoid. To further characterize the intraorganellar location of DegP, intact thylakoids were sonicated and subjected to ultracentrifugation to separate the thylakoid membranes from their soluble lumen contents. DegP was associated exclusively with the thylakoid membrane, with no traces detectable in the lumen, whereas OE33 was equally distributed between the two fractions (Fig. 1B). These results suggested that DegP is strongly associated with the inner side of the thylakoid membrane.
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Expression of Chloroplastic DegP Is Stimulated by Heat-- Bacterial DegP is a heat-shock protein, necessary for survival at elevated temperatures (18). To test the effect of heat on chloroplastic DegP expression, we transferred pea seedlings grown at 25 °C to 40 °C. Increased levels of DegP were observed after 2 and 4 h, with a decrease after longer exposures to high temperature (Fig. 2). The transient increase in DegP levels in response to elevated temperature was in contrast to the constant level of OE33 observed throughout the experiment. Similar to OE33, levels of the stromally exposed thylakoid protease FtsH (24) also remained unchanged (data not shown). Thus, it appears that in addition to a constitutive role, DegP may play a role in the chloroplast's response to transient elevated temperatures.
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Thylakoid Membranes Contain a -Casein-degrading Serine
Protease--
-Casein is the preferred substrate to assay bacterial
DegP activity under in vitro conditions (18). We therefore
tested whether the chloroplast fraction containing the DegP homologue also exhibits
-casein-degrading activity. When thylakoid membranes prepared by sonication followed by centrifugation were incubated with
-casein, >50% of the casein was degraded within the first 60 min
(Fig. 3A). Addition of 0.2%
Triton X-100 only slightly increased the degradation rate. Together
with the aforementioned conclusion that the thylakoid membranes were
for the most part inside-out (Fig. 1C), this suggested that
most of the casein-degrading activity resides on the inner side of the
thylakoid membrane and that no additional molecules of the enzyme are
exposed by solubilizing the membrane.
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A Plant cDNA Encodes a Homologue of DegP--
A search of the
Arabidopsis data base revealed an expressed sequence tag
showing considerable homology to bacterial DegP, including its active
serine region. Since this cDNA was only a partial clone, we used it
as a DNA probe to isolate the full-length homologue from an
Arabidopsis cDNA library. The resultant 1477-base pair-long cDNA, designated AtDegP, encodes a protein of
437 amino acids (Fig. 4), with a
calculated molecular mass of 46,212 Da and a pI of 6.37. The N terminus
of the protein demonstrates the characteristics of a chloroplast
bipartite transit peptide (17). Its stroma-targeting domain, estimated
to be 51 amino acids long, starts with a stretch of 13 residues devoid
of Gly and Pro. It is rich in hydroxylated and basic residues (39 and
10%, respectively) and contains no acidic residues (Fig. 4). Since the
recognition site of the stromal peptidase is only loosely conserved
among different chloroplastic proteins (25), the stromal processing site was not obvious. We predicted it to be either at Ser-43 or at
Ser-51, based on the occurrence of Ile residues at positions 41 and 49, a residue that is often found at position 3 of processed precursors
(25). The stroma-targeting domain is followed by a sequence of at least
52 amino acids, with characteristics of a lumen-targeting domain. It
consists of an N-terminal charged region (rich in acidic residues),
a hydrophobic domain, and a more polar C-terminal region ending with a
recognition site for the thylakoid-processing peptidase
(AXA). The characteristics of the N terminus of the protein
suggested that it serves as a bipartite transit peptide to facilitate
first the import of the protein into the chloroplast and then its
translocation across the thylakoid membrane, consistent with the
immunolocalization of the protein presented in Fig. 1.
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DISCUSSION |
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This study provides the first description of a putative general
purpose protease inside the chloroplast thylakoid. Chloroplastic DegP
is peripherally attached to the inside of the thylakoid membrane, making it available for cleavage of luminal soluble proteins as well as
hydrophilic portions of thylakoid membrane proteins exposed to the
lumen. The localization of DegP to the inner side of the thylakoid is
consistent with the occurrence of its bacterial homologue on the
periplasmic side of the inner membrane (22), with the thylakoid lumen
being considered the functional and evolutionary equivalent of the
bacterial periplasm. In this respect, it is also interesting to note
that members of the -lytic endopeptidase family of serine proteases
have been described only in eubacteria, where they are secreted to act
extracellularly (26).
The DegP-membrane association is fairly strong, as evidenced by its resistance to high salt washes that remove OE33, another peripheral thylakoid membrane protein. Similar resistance to such washes has been observed with bacterial DegP (22). This association appears to be mediated by hydrophobic interactions since it is destabilized by low concentrations of detergent. Hydrophobic interactions between bacterial DegP and the inner membrane can also be implied by the fact that this protein has recently been shown to interact with phospholipid membranes (22). Hydropathy plots of both the Arabidopsis and E. coli proteins did not reveal any hydrophobic sequence long enough to span the membrane (data not shown). However, the occurrence of shorter (~10 residues) hydrophobic stretches may explain their strong interactions with membranes.
Comparison of the amino acid sequence of chloroplastic DegP with the Arabidopsis data base revealed two related genomic clones (F5I14.16 and F5I14.17) found on chromosome 1. These genes were clearly different from the cDNA isolated in this work and are unlikely to encode chloroplastic proteins because they lack putative transit peptides. However, since their N termini are similar to the bacterial signal peptide, they may be translocated through the secretory pathway. Localization of the products of these two genes to cellular sites other than plastids can also be envisioned, as gene homologues of DegP have been recently identified in mammalian cells (27).
Although the physiological substrates of chloroplastic DegP are unknown, one may speculate that it participates in the degradation, or at least partial cleavage, of either soluble or membrane proteins. For example, proteolytic degradation of the photosystem II reaction center D1 protein involves two initial ATP-independent cleavage events in luminal loops connecting transmembrane helices, and the protease(s) involved are of the serine type (for review, see Ref. 28). The possible involvement of DegP in D1 protein degradation awaits direct examination. Efficient degradation of proteins extruding from both sides of the membrane, such as D1, is expected to require protease activity at both membrane surfaces. In this respect, DegP may be an important addition to the FtsH protease found on the stromal side of the thylakoid membrane (24, 29).
Of particular interest was the observation that the steady-state level of chloroplastic DegP increases rapidly upon exposure of seedlings to elevated temperatures. This finding is consistent with the heat-stimulated expression of the bacterial gene (18) and a homologous gene in algae (27). Under these conditions, proteins may undergo conformational changes, resulting in irreversible aggregation. One of the roles of DegP may be to prevent this by degrading heat-denatured proteins in the thylakoid lumen. Our findings provide tools for studying the physiological roles of this newly discovered chloroplastic protease.
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ACKNOWLEDGEMENTS |
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We thank B. Lipinska for the antibody against bacterial DegP, N. Hoffman for the antibody against OE33, and the Arabidopsis Biological Resource Center at Ohio State University for the Arabidopsis expressed sequence tag clone and the cDNA library.
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FOOTNOTES |
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* This work was supported in part by Grant CT940080 from the European Union and the Israeli Ministry of Science (to Z. A.).The costs of publication of this article were defrayed in part by the payment of page charges. The article must therefore be hereby marked "advertisement" in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
The nucleotide sequence(s) reported in this paper has been submitted to the GenBankTM/EMBL Data Bank with accession number(s) AF028842.
Supported by a postdoctoral fellowship from the Federation of
European Biochemical Societies.
§ To whom correspondence should be addressed. Dept. of Agricultural Botany, Faculty of Agriculture, Hebrew University of Jerusalem, Rehovot 76100, Israel. Tel.: 972-8-948-1921; Fax: 972-8-946-7763; E-mail: zach{at}agri.huji.ac.il.
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REFERENCES |
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